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DIAGNOSTIC POTENTIAL OF EXTANT ANTI- 
SCHJSTOSOMA GENUS-SPECIFIC MONOCLONAL 
ANTIBODIES
A Thesis Presented to 
The Board o f  Graduate Studies, 
University o f  Ghana, Legon 
Ghana
In Part fulfilment o f  
the Requirements for the Degree o f  
Masters o f  Philosophy (M. Phil) 
Biochemistry
By
SEFAH KWAME
BSc. (Hons)
Department o f Biochemistry, 
Faculty o f Science, 
University o f Ghana 
Legon, Accra, Ghana.
SEPTEMBER 2001
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I hereby declare that except for the references cited from the work o f other 
researchers, which I have duly acknowledged, this work was as a result of my own original 
research and this thesis, either in whole, or in part has not been presented for another 
degree elsewhere.
DECLARATION
KWAME SEFAH 
(Student)
A
Dr. K. M Bosompem 
(Supervisor)
Prof. F. N. Gyang 
(Supervisor)
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DEDICATION
To my wife 
And 
Children
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I am greatly indebted to my supervisors Dr. K. M. Bosompem o f the Noguchi 
Memorial Institute for Medical Research (NMIMR) and Prof. F. N. Gyang, Department o f 
Biochemistry, University o f Ghana. This thesis could not have been completed without 
their forbearance, patients, expert guidance and constructive comments. I am also grateful 
to the Director o f  NMIMR Prof. D. Ofori-Adjei and the entire staff o f  the Institute for the 
assistance offered me. I am especially thankful to the head o f  the Parasitology Unit, Dr. 
M. D. Wilson for accommodating and encouraging me throughout my stay at the Institute. 
The contributions o f  Mr. M. A. Appawu, Dr. D. Boakye and Dr. Y. Osada (JICA expert) 
were tremendous.
I am also exceedingly grateful to the following Mr. W. K Anyan, J. Otchere, U. S. 
McKakpo, D. Boamah, J. Quartey, J. R. K. Asigbee, S. K. Dadzie, S. Otoo, Mrs. I. Ayi all 
o f the Parasitology Unit for their encouragement likewise Mr. E Asiedu-Opare, Aggoe 
(Drivers) for taking me to and from the field. In addition the assistance o f the following 
was remarkable, Mr. H. Asmah, Odoi, and Sis. Susie o f the Electron Microscopy Unit as 
well as the entire staff o f  the P3 laboratoiy for assisting me in the use o f some facilities, 
particularly the computarised Microplate plate reader.
I am also very grateful to all the lecturers at the Department o f  Biochemistry, 
University o f Ghana, for the training and the discipline that they have instilled in me.
The following people have also contributed immensely in diverse ways, Mr. 
Solomon Yaw Darko, Mrs. Annis Darko Mr. John Dadzie Mensah, Justice Essoun-Nyarko 
and Banson Richard.
To all my family members especially, Messers Anane Boateng, Kofi Duah, J. S. 
Adu-Sefah, Mrs. Mercy Adu-Sefah and Kwasi Addai for their prayers and financial 
support and to my wife Vivian Anowi and my children Adelaide Sefah, Kofi Sefah and 
Nana Amma Sefah-Antwi, I say God Bless you all for you patience.
ACKNOWLEDGEMENT
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I again wish to thank the people o f Galilea and Agbekotsepko for providing me 
with specimen for the entire project.
Finally, I acknowledge the financial support o f  this project by Shell Ghana Limited, 
which provided a student stipend.
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TABLE OF CONTENTS
DECLARATION...........................................................................................................................1
DEDICATION.............................................................................................................................n
ACKNOWLEDGEMENT.......................................................................................................HI
TABLE OF CONTENTS...........................................................................................................V
LIST OF TABLES...................................................................................................................VH
LIST OF FIGURES...............................................................................................................VID
LIST OF PLATES........................................................................- ..........................................IX
LIST OF ADDREVIATIONS.................................................................................................. X
ABSTRACT...............................................................................................................................XH
CHAPTER 1............................................................................................................................... - 1
INTRODUCTION AND LITERATURE REVIEW ................................................ - ..........1
INTRODUCTION......................................................................................................................1
Objectives o f  the study......................................................................................................... 4
Justification for the study......................................................................................................4
LITERATURE REVIEW......................................................................................................... 5
Schistosomiasis and Schistosomes...................................................................................... 5
The S. haematobium group .............................................................................................. 6
The S. mansoni group ....................................................................................................... 7
The S. indicum group........................................................................................................8
The S. japonicum group ....................................................................................................9
The life cycle o f  schistosomes........................................................................................10
Schistosomiasis in Ghana...................................................................................................15
Animal schistosomiasis...................................................................................................... 17
Schistosome antigens.......................................................................................................... 20
Adult Worm Antigen (AWA)............................................................................................20
Schistosomula Surface Antigen........................................................................................ 21
Schistosome Egg Antigens (SEA)..................................................................................23
Cross- reactive Antigens................................................................................................ 24
Excretory-secretory Antigens.........................................................................................25
Enzyme-linked Immunosorbent Assay (ELISA).............................................................26
Monoclonal Antibodies (MoAbs)..................................................................................... 27
Uses o f  Antibodies..........................................................................................................29
Purification o f  Antibodies..............................................................................................29
Diagnosis o f  human schistosomiasis.................................................................................31
Eggs in urine................................................................................................................... 31
Eggs in Stool................................................................................................................... 32
Biopsies............................................................................................................................ 33
Immunodiagnosis............................................................................................................ 33
Diagnosis o f  animal schistosomiasis.................................................................................36
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CHAPTER 2 37
GENERAL MATERIALS AND METHODS......................................................................37
Study area ............................................................................................................................ 37
Resuscitation o f Hybridoma Cells..................................................................................... 37
Cloning and Propagation o f  Hybridoma Cells................................................................. 38
Cryopreservation o f  Hybridoma Cells...............................................................................39
Determination o f Immunoglobulin Class and Subclass..................................................39
Purification o f  Monoclonal Antiboddies..........................................................................40
Amicon Filtration............................................................................................................40
Ammonium Sulphate Precipitation................................................................................40
Gel Filtration.................................................................................................................. 40
Micro-Plate ELISA..............................................................................................................41
Cross-reactivity testing o f  MoAbs using schistosome and P. falciparum antigens in
microplate ELISA...............................................................................................................42
Preparation o f Horseradish Peroxidase Antibody Conjugates....................................... 42
Coating o f the Test MoAbs on PVDF and Nitrocellulose Membranes by Dot-ELISA
............................................................................................................................................... 43
Coating o f the Selected MoAbs to Micro-titre Plates.....................................................44
Dipstick ELISA procedure................................................................................................. 45
Microplate-based Sandwich ELISA..................................................................................45
Membrane-based sandwich ELISA...................................................................................46
Microscopical Diagnostic Methods...................................................................................46
Collection and Analysis o f  Human Urine and Stool Specimen..................................46
Collection and Analysis o f  Cattle Blood and Faecal Samples...................................47
Fixation o f  miracidia with Kamovsky reagent................................................................48
IF AT Procedure................................................................................................................... 48
CHAPTER 3 .......   49
RESULTS................................................................................................................   49
Prepared monoclonal antibody reagents...........................................................................49
Reactivity o f selected monoclonal antibodies as determined by micro-plate ELISA. 52
Development o f  assays.......................................................................................................59
Detection o f  Schistosoma antigens in human urine using the selected monoclonal
antibodies.........................................................................................................................59
Prevalence o f  Schistosoma infection in cattle as determined by microscopy..............66
Schistosoma infection rates in cattle as determined by IF AT and micro-plate ELISA 
...............................................................................................................................................69
CHAPTER FOUR..............................................................................................................  71
DISCUSSION AND CONCLUTION....................................................................................71
REFERENCES...........................................................................................................................78
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Table 1. Some biological characteristics o f  the selected monoclonal
antibodies.........................................................................................................50
Table 2. Reactivity o f  the selected monoclonal antibodies........................................ 53
Table 3. Prevalence o f  urinary and intestinal schistosomiasis as determined
by microscopy and dipstick-ELISA using different MoAbs....................61
Table 4. Diagnosis o f  schistosomiasis by microscopy and dipstick-ELISA
using the selected MoAbs.............................................................................62
Table 5. S. haematobium egg count............................................................................. 63
Table 6. Binding studies o f the selected MoAbs onto different micro titre
plates and membranes.................................................................................... 65
Table 7. Detection o f parasite ova in stool samples o f cattle (short horn variety)
from Agbekpotsepko.................................................................................... 67
Table 8. Diagnosis o f  schistosomiasis in cattle by microscopy and micro-plate
ELISA using the selected MoAbs.................................................................70
LIST OF TABLES
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Figure 1. Reactivity o f  Sh3/34.10 with schistosome antigen and P. falciparum
crude antigen extract.................................................................................... 54
Figure 2. Reactivity o f  Sh3/38.2 with schistosome antigen and P. falciparum
crude antigen extract.................................................................................... 55
Figure 3. Reactivity o f  Sh4/14.3 with schistosome antigen and P. falciparum
crude antigen extract.................................................................................... 56
Figure 4. Reactivity o f  Sh5/32.30 with schistosome antigen and P. falciparum
crude antigen extract.................................................................................... 57
Figure 5. Reactivity o f  Sh5/34.10 with schistosome antigen and P. falciparum
crude antigen extract.................................................................................... 58
LIST OF FIGURES
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Plate 1. Immunodiffusion............................................................................................ 51
Eggs o f  parasites identified in faecal specimen o f cattle 
Plate 2. S. bovis............................................................................................................68
LIST OF PLATES
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ABBREVIATIONS
ABTS Azino-bis(3-ethylbenzthiazoline-6-sulfbnic acid)
DAB Diaminobenzidine tetrahydrochloride
DMSO Diamthylsulfoxide
EDTA Ethylenediaminetetraacetate
ELISA En2yme-linked immunosorbent assay
FBS Foetal bovine serum
FITC flourescein isothiocynate
Hr Hour
HRPO Horseradish peroxidase
IFAT Indirect immunoflourescent antibody test
Ig Immunoglobulin
IgA Immunoglobulin A
IgD Immunoglobulin D
IgE Immunoglobulin E
IgG Immunoglobulin G
IgM Immunoglobulin M
1 Litre
MoAb Monoclonal antibody
ml Millilitre(s)
min Minutes
Mr Molecular weight
fi) Microlititre
\ig Microgramme
NMIMR Noguchi Memorial Institute for Medical Research
PBS Phosphate buffered saline
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PH Negative logarithm base o f hydrogen ion concentration
TBS Tris buffered saline
Xg Times gravitational force
ABTS 2,2-azo-bis-3-ethylbenzthiazoline-6-Sulphonic acid
OPD O-phenylenediam ine
TMB 3,3’ 5,5’-tetramethylbenzidine base
pNPP p-nitro phenylphosphate
IMDM Iscove’s Modified Dulbecco’s Medium
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ABSTRACT
The suitability o f  five Schistosoma genus-specific monoclonal antibodies (MoAbs) 
(Sh3/34.10, Sh3/38.2, Sh4/14.3, Sh5/32.30 and Sh5/34.10) in detecting schistosome 
antigens in infected human and cattle was evaluated. These antibodies were employed in 
various diagnostic assays to diagnose human and animal schistosomiasis. Extant MoAb 
secreting hybridoma cells were first propagated in culture to produce the MoAbs. The 
culture supernatants containing secreted antibodies were analysed by immunodiffusion and 
the isotypes o f  the immunoglobulins shown to be IgM (Sh3/34.10, Sh3/38.2, Sh5/32.30 
and Sh5/34.10) and IgGl (Sh4/14.3). Gel purified fractions o f  the MoAbs were utilised in 
developing dipstick ELISA and micro-plate ELISA in diagnosing schistosomiasis. Also, 
the suitability o f  the indirect immunoflourescent Antibody Test (IFAT) was employed to 
demonstrate anti-schistosoma antibodies in the blood o f infected cattle.
Three o f  the antibodies (Sh3/38.2, Sh4/14.3, Sh5/32.30) showed no cross-reactivity 
with Plasmodium falciparum  circum-sporozoite protein (CSP) and crude antigen extract of 
P. falciparum. However Sh3/34.10 and Sh5/34.10 reacted with the crude antigen extract 
o f P. falciparum  at high antibody concentrations even though the reactivity was abrogated 
at higher antibody titres.
In human schistosomiasis, the diagnostic potential o f  the MoAbs in detecting 
schistosome antigens were assessed alongside microscopy and the standard Sh2/15.F 
urinary schistosomiasis dipstick ELISA developed by researchers at the NMIMR. Out o f 
74 human subjects from a schistosomiasis endemic area screened for urinary 
schistosomiasis, 81.1% were microscopically positive for S. haematobium eggs whilst the 
standard dipstick assay gave prevalence estimate o f 87.3%. The sensitivity o f this assay 
was 100% whereas the specificity was 64.7% compared with microscopy as the gold 
standard test. Dipstick assays utilizing the individual Schistosoma genus-specific 
monoclonal antibodies estimated prevalences o f  urinary schistosomiasis between 48.6 and
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58.1%. The sensitivities o f the assays were however lower (60.0-71.1%) compared with 
microscopy as the gold standard test. Nonetheless, each o f the antibodies showed a high 
specificity o f  100% in detecting S. haematobium urinary antigens. The Schistosoma 
genus-specific antibodies performed similarly when utilized in dipstick to detect S. 
mansoni infections.
Two assays (IFAT and MoAb-based plate ELISA) were developed to diagnose 
animal schistosomiasis in cattle. The sensitivities o f  these assays compared well with 
microscopy. In determining the prevalence o f S. bovis, microscopy gave a prevalence o f 
53.1% compared with 50.0% determined by IFAT. Micro- plate based ELISA utilizing 
different Schistosoma genus-specific MoAbs estimated prevalence o f S. bovis between 
46.9% and 50.0%. These assays were sensitive (ranging from 88.2-94.1%) compared with 
microscopy as the gold standard test and the specificity was each 100%. In view o f  the 
limitations o f the microscopical approach the assays provided alternative diagnostic tool in 
detecting animal schistosomiasis in cattle.
The study also demonstrated 3.1% (1/32) prevalence o f S. indicum in mixed 
infection with S. bovis by microscopy. Eleven other cattle parasites eggs were 
demonstrated by microscopy with prevalence ranging from 3.1-21.9%. There was no 
evidence o f  cross-reactivity between the antigens o f these parasites and the Schistosoma 
genus-specific MoAbs utilised.
This study revealed the diagnostic potentials o f  the Schistosoma genus-specific 
MoAbs in detecting schistosome antigens in both humans and cattle. The development of 
Schistosoma genus-specific MoAb-based dipstick ELISA for diagnosing schistosomiasis is 
promising.
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CHAPTER 1
INTRODUCTION AND LITERATURE REVIEW 
INTRODUCTION
Schistosomiasis is the name given to the group o f  human and animal diseases 
caused by blood-dwelling helminth o f  the genus Schistosoma. Schistosomiasis infections 
are normally chronic and take many years. Despite the availability o f  chemotherapy, more 
than 200 million people and millions o f  domestic animals are infected with schistosomes in 
73 countries that harbour the intermediate snail host o f  the family Planorbidae (Manson- 
Bahr and Bell, 1991). In addition, 600 million people are at risk o f  infection. The affected 
areas include Africa, South America, India, South-East Asia, the Far East, part o f  the 
Middle East and the Mediterranean countries including a small focus in Portugal 
(Rollinson and Southgate, 1987). The World Health Organisation (W.H.O) reports that 
schistosomiasis is second most prevalent parasitic disease in the tropics after malaria 
(Atlas, 1995).
Three main species o f schistosomes (Schistosoma mansoni, S. japonicum  and S.
haematobium) are responsible for infection in humans (Boothroyd and Komuniecki, 1995).
However the contributions o f  other species such as S. mekongi and S. intercalatum cannot
be underestimated. A number o f species are also known to infect livestock. These
include: S. matheei (commonly in cattle, sheep and goat); S. bovis (cattle); S  leiperi
(herbivores); S  indicum (variety of domesticated animals including sheep camel goat and
cattle) and S. spindale (ruminants) (Rollinson and Southgate, 1987). Schistosomiasis is
primarily a rural disease whose transmission depends on a variety o f  factors including; (1)
contamination o f fresh water with human/animal urine or faeces containing viable
Schistosoma eggs, (2) the presence o f schistosomiasis host snails and in the case o f aquatic
species, water temperature, rate o f  flow, acidity or alkalinity and the content o f  organic
matter conducive to snail growth are important factors and (3) human contact with water
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containing infective cercariae (Manson-Bahr and Bell, 1991). Infection with 
schistosomiasis is initiated when cercariae penetrate the skin and transform into 
schistosomula, which subsequently enter the vasculature and migrate via the lungs to the 
hepatic portal system (S. mansoni and S. japonicum ) or the urogenital venules (S. 
haematobium) (Boothroyd and Komuniecki, 1995). In some parts o f Africa, where S. 
haematobium and S. mansoni are prevalent, mixed infections are common. Manson-Bahr 
and Bell (1991) reported 60% mixed infections in parts o f the Nile Delta and 22% in 
European patients in Zimbabwe.
Typically in areas endemic for Schistosomiasis, the distribution o f infection 
intensity is overdispersed, such that younger people (less than 18 years old) excrete more 
eggs and therefore are more heavily infected than older individuals (Boothroyd and 
Komuniecki, 1995). Following chemotherapy, re-exposure to infective cercariae leads to 
rapid re-infection in young people who may regain heavy infection whereas older 
individuals tend to be less severely affected.
A definitive diagnosis of schistosomiasis may be achieved by examination o f the 
urine, stool, rectal or bladder biopsy for eggs through microscopy and also by serological 
tests. The microscopical technique, which is the most commonly used, is very specific 
(100%) but not sensitive enough. Moreover it is time consuming, tedious and not field 
applicable making its dependency limited. There is therefore the need for differential 
diagnosis. The Serological tests (based on the detection o f host antibodies directed against 
schistosome antigen) on the other hand are useful in diagnosis o f  both apparent and 
inapparent infections. Virtually all the well-established assays including Enzyme-linked 
immunosorbent assay (ELISA), Indirect Immunofluorescence assay, Slide flocculation, 
Plasma card, Precipitin, Indirect Haemagglutination, Miracidial immobilization, 
Circumoval precipitin test (COPT) and Complement fixation test (CFT) (Manson- Bahr 
and Bell, 1991), have been applied to identification of schistosome species and the
diagnosis o f schistosomiasis, however, very few have been advocated for large-scale use in
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diagnosis due to lack o f  sensitivity. Among the most promising alternative diagnosis for 
urinary schistosomiasis are the Schistosoma genus- specific circulating anodic and 
cathodic antigen (CAA and CCA) detection assay (Kremsner el al., 1994; De Jonge et al., 
1989) and the recently developed S. haematobium species-specific dipstick ELISA 
(Bosompem et al., 1996a). These are more sensitive and detect circulatory and or urinary 
antigens utilizing non-invasive membrane-based assays, which are more suited for field 
use in endemic areas. The CAA and CCA detection assays are yet to be adopted for use. 
On the other hand, the urinary schistosomiasis dipstick has been tested in some parts o f 
Ghana and successfully adopted for application in routine diagnosis o f  the disease in the 
field. The specific detection o f S. mansoni is yet to be developed.
The incidence o f  mixed infections limits the extent o f  the applicability o f the 
urinary Schistosoma dipstick method in diagnosis because positive test results are silent on 
the mixed infections o f  S. haematobium with other schistosome species. There is thus the 
need to develop field applicable assays, which are either S. mansoni species-specific or 
Schistosoma genus-specific so that other schistosome infections and or mixed infections 
could be diagnosed. In circumstances where the urinary Schistosoma dipstick is used 
alongside a Schistosoma genus-specific assay in humans, intestinal schistosomiasis may be 
diagnosed by exclusion. It was for these reasons that the present study was conducted to 
determine the diagnostic potential o f  existing Schistosoma genus-specific monoclonal 
antibodies and further utilised in the development o f membrane/micro-plate based 
ELISA’s for the diagnosis o f both human, and animal schistosomiasis, which has little 
attention.
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Objectives of the study
(i) To produce monoclonal antibodies in vitro by propagating existing hybridoma cells
and purifying the antibodies for use in diagnosis.
(ii) To determine the specificity o f purified monoclonal antibodies in cross-reactivity
studies using crude antigen extracts o f  S. haematobium, S. mansoni, S. japonicum, 
and Plasmodium falciparum..
(iii) To utilize Schistosoma genus-specific monoclonal antibodies in developing 
membrane or micro-plate based ELISA for diagnosis o f schistosomiasis.
(iv) To diagnose S. mansoni infection in humans by exclusion using the developed
Schistosoma genus-specific ELISA and the existing S. haematobium species- 
specific dipstick method. ELISA.
(v) To utilize the developed Schistosoma genus-specific monoclonal antibodies in
detection o f  schistosome antigens in infected animals using blood specimens.
(vi) To determine the specificity and sensitivity o f the Schistosoma genus- specific
monoclonal antibody-based assays by comparison with the microscopical detection 
o f parasite ova in urine and stool specimens.
Justification for the study
The determination o f the diagnostic potential o f  Schistosoma genus-specific 
monoclonal antibodies would promote accurate diagnosis o f  mixed schistosome infections 
in humans. Also the establishment o f  field applicable Schistosoma genus-specific 
diagnostic assays would enable investigations into the occurrence and spread o f  animal 
schistosomiasis in Ghana on which currently there is little, if any, information available.
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LITERATURE REVIEW
Schistosomiasis and Schistosomes
Schistosomes are trematodes belonging to the family Schitosomatidae. Members 
o f  this family show morphological and physiological peculiarities, which set them apart 
from other trematodes. They are dioecious digenia. The male worm is flat and leaf-like 
and is folded to form a gynaeocophoric canal formed by ventrally flexed lateral outgrowths 
where the slender female is held (Manson-Bahr and Bell, 1991; Rollinson and Southgate, 
1987).
Schistosomes live in the blood stream o f warm-blooded hosts, being the only 
trematodes to do so. The specific location o f the parasite in the host depends on which 
schistosome species is involved. For instance S. haematobium localises in the vesical 
plexus around the urinogenital system whilst S. mansoni, S.japonicum, S. intercalatum and 
S. mekongi are normally found in the hepatic portal system around the gastro-intestinal 
tract (Sturrock, 1993).
The life cycle o f  schistosomes consists o f  alternate generations, each with its own 
host. The adult worms infect vertebrates and the two larval stages miracidia and cercaria 
occur in susceptible snail. Miracidia hatch from the eggs and invade the snails specific to 
each schistosome species whilst the cercaria leave the snail to invade definitive host. A 
feature o f  the life cycle o f  schistosomes is that multiplication takes place in each o f the 
different hosts so that it is very difficult to break the cycle (Manson-Bahr and Bell, 1991).
The family schistosomatidae is divided into three subfamilies, the
Schistosomatinae, Bilharziallinae and Gigantobilharzianae (Rollinson and Southgate,
1987), consisting o f twelve genera in all. Seven out o f these genera are confined to birds
and the rest to mammals. However, only the genus Schistosoma is associated with man
(Rollinson and Southgate, 1987). This genus has achieved the greatest geographical
distribution and diversification in terms o f numbers o f  recognised parasite species and
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different hosts parasitised. The overall distributional range o f the different schistosome 
species is primarily influenced by the presence or absence o f  suitable mammalian and 
intermediate snail host (reviewed by Sturrock 1987). Some schistosomes easily infect 
snail o f one geographical area but fail to infect or infect with difficulty the same snail from 
a different area (Manson-Bahr and Bell, 1991). The genus Schistosoma is recognized by 
eighteen species placed in four different groups also called species complexes by Kuntz 
(1955). This was based on the common relationships o f the parasite species within 
particular snail host genera and on zoo-geographical distribution pattern as well as the 
morphology o f the parasite eggs. The groups are the S. haematobium, S. mansoni, S. 
japonicum  and S. indicum species complexes.
The S. haematobium group
Schistosoma haematobium was the first schistosome to be described. Bilharz 
identified the parasites in 1852 and in 1864 Harley reported urinary schistosomiasis in 
people in South Africa (Rollinson and Southgate, 1987; Sturrock, 1993). The S. 
haematobium group is widely distributed in Africa and the Eastern mediterranean region 
including Iran, Islamic Republic o f Iraq, Jordan, Lebanon, Oman, Saudi Arabia, Syria and 
Yemen (Sturrock, 1993). The species complex consists o f  seven species. These are S. 
haematobium, S. intercalatum, S. metheei, S. bovis, S. carassoni, S. margrebowiei and S. 
leperi. Members within the group show substantial dissimilarities in the morphology of 
the egg as well as the definitive host specificity. There is thus evidence for geographical 
variation in many characters associated with the S. haematobium group o f species. For 
example, studies by Wright and Knowlers (1972) on laboratory hamsters showed that 
differences occur between geographical strains o f  the parasite in many biological features 
such as intermediate host specificity, infectivity o f cercariae, growth rates and maturation 
times o f adult worms, fecundity rate and host-organ distribution o f eggs. In general the
intermediate host o f  S. haematobium species complexes are the Bulinus species. S.
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haematobium in the Afrotropical region is transmitted by snails o f the B. africanus group, 
whilst in the Mediterranean area and S. W. Asia it is by tetraploid members o f  the B. 
truncat us/tropicus complex. In Arabia and Mauritius transmission is by members o f  the B. 
forskalii group. In West Africa, however, all the three snail groups are known to act as 
intermediate hosts for S. haematobium (Frendson, 1979). O f particular significance is the 
division between S. haematobium from North Africa and the Middle East, and the parasite 
from the Afrotropical region. With few exceptions, neither o f  the parasites can develop in 
the snail host o f the other.
Though there are marked differences between members o f the S. haematobium 
group, natural hybridisation has been reported to occur. For example a Camerounian strain 
o f  S. haematobium and S. intercalatum hybrid was reported from Loum, in a previously 
‘pure’ S. haematobium area (Jordan and Webbe, 1993). Again, ample evidence has 
accumulated from different sources with various reports o f  the occurrence o f natural 
hybrids o f S. haematobium and the cattle parasite S. metheei in humans (Van Wyk, 1983).
The S. mansoni group
Intestinal schistosomiasis in man is mainly caused by S. mansoni, the schistosome 
species with considerable amount o f  information (Rollinson and Southgate, 1987). The 
early stages o f  chronic infections are free o f  obvious symptoms and signs but the later 
stages, with liver and spleen enlargement, are more easily detected by clinical examination 
(Jordan and Webbe, 1993). The parasite is common in Libya, Oman, Saudi Arabia, 
People’s Democratic Republic o f Yemen, Madagascar and over greater part o f  Africa 
south o f the Sahara. In the Carribbean it is endermic in Puerto Rico, Saint Lucia, Antigua, 
Dominican Republic, Martinique and Montserrat. Several reports o f infection with S. 
mansoni in a wide array o f  mammalian hosts have been made. The role o f animal hosts in 
maintaining the parasite has also been reported. For instance, Fenwick (1969) recovered 5.
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mansoni from all seven baboons examined in an area o f  Northern Tanzania, particularly 
uninhibited by man.
Experimental evidence has shown that S. mansoni strains from different 
geographical areas may display differences in their biological characteristics and in their 
infectivity or pathogenicity. For instance, de Lima e Costa and Katz (1982) observed that 
in mice, strains o f  S. mansoni originating from the same locality may show statistical 
differences in infectivity, effect on leucocyte count, numbers o f eggs per female worm and 
response to treatment. Other members o f the species complex include S. edwardiense and 
S. hippopotami, both o f  hippopotamus (Rollinson and Southgate, 1987), and S. rodhaini 
found in dogs, civic cat as well as a variety o f rodents. The major intermediate hosts are 
the group o f  snails o f  the genus Biomphalaria. Almost all known species are susceptible 
to S. mansoni.
The S. indicum group
Members o f  this species complex are mostly o f  veterinary importance. S. indicum, 
first reported in equines by Montgomery (1906) is known to infect a variety o f 
domesticated animals on the Indian subcontinent including sheep, camel, goat, cattle and 
buffalo. Another member S. spindale is found in the portal and mesenteric veins o f the 
small and large intestine o f ruminants. The parasite has been reported in many parts o f 
India, Sri Lanka, Indonesia, Malaysia, Thailand and Vietnam. It is also thought to be one 
o f  the causes o f  schistosomal dermatitis in man, especially in rice paddy fields where S. 
indicum infected buffaloes coexist with the intermediate host Indoplanobia exustus. The 
rodent Bandicota bengalensis has been found naturally infected with S. indicum (Rollinson 
and Southgate, 1987).
Another member, o f  the S. indicum group, Schistosoma nasale is responsible for 
nasal schistosomiasis, or snoring disease in cattle, sheep and goats. The adult worms are
found in the veins o f  the nasal mucosa. Also, S. incognitum, is reported in Thailand, Java
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and Sulamesi primarily in rodent species o f  the genera Bandicota and Rattus, and in wild 
deer in Indonesia. In India, it is commonly found in pigs. In Thailand and Indonesia, 
Radix auricularia appears to be the intermediate host o f  S. incognitum (Rollinson and 
Southgate, 1987).
The S. japonicum group
Schistosoma japonicum  differs from the other schistosome species affecting man in 
many ways. Probably, the greatest significance is the acute stage o f its infection, a well 
recognised and frequently fatal condition that can be o f epidemic proportion (Jordan and 
Webbe, 1993). It is responsible for a grave, debilitating and chronic form o f intestinal 
schistosomiasis, which affects both man and domestic animals. It has a reputation o f being 
the most serious o f  the schistosomes affecting man, generally because o f the large number 
o f  eggs produced by the adult female worms. The disease in the Far East is endemic in 
parts o f  China (Hunan, Hubei, Jiangxi, Anhui and Jiangsu Provinces) (Yuan Hong, 1993), 
Phillipine, Japan (Kufu, Katayama and Chikugo River Basin), Taiwan and Indonesia. 
Schistosoma japonicum  occurs as a natural parasite o f  a large number o f  mammalian 
species, which play an important role in the epidemiology o f  the disease. In some endemic 
areas in Mainland China, 31 species o f wild animals including carnivores, rodents, 
primates, insectivores and artiodactyls have been found with natural infections o f S. 
japonicum  (Mao and Shao, 1982). All the strains of S. japonicum  are transmitted by 
populations o f  the amphibious polytypic snail Oncomelania hupensis which consists o f six 
subspecies. These are O. h. chiui and O. h. formosana in Taiwan, O. h. hupensis in 
Mainland China, O. h. lindoensis in Sulamesi, O. h. quadrasi in the Philippines and O.h. 
nosophora in Japan (Davis, 1980). Other group members include S. mekongi and S. 
sinensium. S. mekongi is responsible for human schistosomiasis in Khong Island in the 
Mekong River in Southern Laos and in many parts o f  northern and central Kampuchea
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(Cambodia) (Voge et al., 1978). The intermediate host is Tricula aperta (Liang and 
Kiticoon, 1980).
The life cycle o f schistosomes
Though the first schistosome was described in 1851 by the German pathologist 
Theodor Bilharz, it was not until 1915 that the life cycle o f  the schistosomes was 
unraveled. This revealed the connection between the diseases and the fresh water 
planorbid snail which act as intermediate host to the parasites (Rollinson and Southgate, 
1987). The life cycle comprises o f  the following stages; egg, miracidium, first and second 
stage sporocysts, cercaria, schistosomulum and adult worm. The first and second stage 
sporocysts reproduce asexually within the snail whilst the adult worms reproduce sexually 
in the definitive mammalian host.
The eggs laid by schistosome worms in the definitive mammalian host are passed 
out into fresh water via the urine or stool depending on the species o f  schistosome. In 
water, the eggs hatch into the first larval stage, the miracidium (Manson-Bahr and Bell, 
1991). For instance S. haematobium eggs are mostly passed through urine (though not 
exclusive) whilst S. mansoni, S. japonicum, S. matheei and S. intercalatum eggs are 
released mostly through faeces. There is a wide range o f size and shape o f  the schistosome 
eggs and the shape has been found to vary with the parasite species and diet o f  the 
definitive host (Rollinson and Southgate, 1987). The eggs are non-operculate, round or 
oval with one spiny appendage (Manson-Bahr and Bell, 1991), found in lateral or terminal 
position. This character o f the eggshell is a very important distinguishing feature o f  one 
schistosome species from another on morphological basis. Schistosome eggs secrete 
histolytic enzymes through micropores in the shells, which help passage through the 
endothelium o f the blood vessels. It is the soluble egg antigens, mostly the charbohydrate 
component) which is responsible for much o f the pathology (Manson-Bahr and Bell, 1991;
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Sturrock, 1993). The embiyo within the egg develops into the next larval stage, the 
miracidium.
The miracidium has a complex array o f  sensory receptors, which are considered to 
aid in locating a snail host. It is thought that miracidia are attracted to intermediate snail 
host by undefined complex o f water-soluble substances (miraxone) secreted by the snails. 
This has been confirmed by the attraction o f S. mansoni miracidia to B. glabata (Chemin, 
1970) and S. haematobium miracidia to B. globosus (Shiff and Kriel, 1970). Miracidium 
swims actively by means o f  its ciliated epidermis, which beat rhythmically to propel it to a 
compatible snail host. It must be emphasized that miracidia do not discriminate between 
species o f  snails and will sometimes enter the incorrect host thereby preventing further 
development (Manson-Bahr and Bell, 1991). However, if a miracidium enters a 
compatible intermediate host, it metamorphosis into the next stage, the mother sporocyst.
The penetration occurs by a mechanical action o f  the apical papilla breaking the
snail’s epithelium while the numerous membrane folds o f  the terebratorium act as a sucker
to facilitate fixation as revealed by light and electron microscopy (Kinoti, 1971; Brooker,
1972; Lo Verde, 1975). The ciliated epidermis o f  the mother (primary) sporocyst is cast
off and is replaced by a syncytial tegument. Within the elongated sac o f the mother
sporocyst, germinal cells develop into a number o f daughter sporocysts. These leave the
mother sporocyst after about 8 days and migrate to the digestive gland (liver) o f the snail
host (Manson-Bahr and Bell, 1991; Sturrock, 1993). Within them further germinal cells
develop asexually into numerous biforked-tailed free-swimming cercariae. The mature
cercaria escapes from the daughter sporocyst, migrates through the tissue o f  the snail and
finally emerges to swim freely in the water by means o f its muscular, bifurcated tail.
Thousands o f  cercariae o f  the same sex may be developed from one miracidium. Cercariae
are unisexual, non-feeding, fish-like with a pear-shaped head. They depend entirely on
their glycogen reserves (Wilson, 1987) and are influenced by light, gravity agitation, touch
and temperature. They are therefore short lived (Manson-Bahr and Bell, 1991). It is the
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second free-living infective schistosome larva. Cercariae o f  all human schistosomes are 
grossly similar, about 1mm in length. The oral head has an anterior sucker (Cousin and 
Dorsey, 1991) and a prominent, muscular ventral sucker or acetabulum, a mouth, 
oesophagus and a pair o f  short caeca. It also has an excretory system o f  flame cells, 
tubules and excretory ducts leading into an excretory bladder at the posterior end o f  the 
body. Electron microscopy has revealed that the body is covered by a tegument bounded 
by a lipid bilayer, which appears trilaminate, usually covered by an amorphous glycocalyx 
(Sturrock, 1993). They tend to accumulate in the area o f the mantle collar o f  the snail, that 
is, close to the head o f  the snail in the region where escape to the outside is simple.
The pattern o f  the release o f  cercariae differs somewhat between the three main 
human schistosomes. Normally S. mansoni cercarial shedding starts within 1 to 2 hours 
after stimulation. The process is more prolonged for S. haematobium, which takes 2 to 4 
hours. Pesigan el al. (1958) reported that the process was even slower for S. japonicum  
requiring many hours o f  stimulation before shedding.
The life cycle is continued if  a cercaria penetrates the intact skin o f man or 
subcutaneous tissue into the blood circulatory system (Sturrock, 1993). Three distinct 
phases have been described by Haas and Schmidt (1982) to be involved in penetration. 
These are (1) attachment; (2) creeping over surface exploring for an entry site and (3) 
penetration into the epidermis. Phases 1 and 2 can be stimulated by thermal and chemical 
stimuli whereas phase 3 is stimulated by chemical stimuli alone. Haas and Schmidt (1982) 
further demonstrated that only aliphatic hydrocarbon chains with both a polar and a non­
polar head group were effective stimulants. Free fatty acids produced on human skin by 
the action o f  bacterial esterases on triglycerides are thought to be the probable natural 
stimulants (Rollinson and Southgate, 1987).
Penetration o f  the cercaria is the result o f  coordinated muscular and secretory
processes in the cercaria, presumably under nervous control. Following entry, the cercaria
transforms into a tailless worm-like schistosomulum before entering the blood system
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directly (or rarely, indirectly via the lymphatics) to be carried passively via the right heart, 
lungs and left heart to the general systemic vessels. It then enters the splanchnic blood 
vessels en route to the liver and matures into adult worm (Sturrock, 1993). Most worms 
leave the liver when they are sexually mature and have mated. They then migrate to the 
veins o f  the vesical plexus (S. haematobium) or the mesenteric veins (S. mansoni, S. 
japonicum, S. metheei and S. intercalatum) where they begin to lay eggs. The period 
between penetration by the cercaria and egg laying may be 30-50 days or more (Manson- 
Bahr and Bell, 1991).
The transformation from cercariae to schistosomulum involves profound 
morphological and physiological changes. The cercarial glycocalyx is lost during this 
period and the single bilipid epithelial membrane surrounding the body is replaced by a 
double bilayer that appears as a heptalaminate membrane in electron micrographs. The 
two lipid bilayers are linked by larger protein molecules detected by freeze-fracture 
ultramicroscopy (McLaren, 1980). A fully transformed schistosomulum has obvious oral 
and ventral suckers and is elongated posteriorly compared with the cercarial body as 
revealed by ultrastructural studies on the transformation process by Basch and Samuelson, 
(1990).
Cercaria as well as young schistosomulum, o f  3-4 hours are susceptible to killing 
by eosinophils, neutrophils and macrophages (McLaren and Ramalho-Pinto, 1979; 
McLaren and James, 1985). They are fully susceptible to complement (C) damage either 
by the alternate or by the classical pathways (Fishelson, 1989). However, during 
development, schistosomulum acquires resistance to complement-mediated damaged 
(Levi-SchafFer et al 1982; Marikovsky et al., 1986;). This conversion to C-resistance 
occurs both in vitro and in vivo upon incubation in artificial medium (Clegg and Smither, 
1972; Fishelson, 1989; Horta et al., 1991). The parasite also adapts to the isotonic medium 
within the definitive host (Sturrock, 1993; Tarrab-Hazdai et al., 1997).
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The adult worm (male and female) has a prehensile oral sucker, which surrounds 
the mouth anteriorly, and a ventral sucker on the ventral surface. The worm attaches itself 
to the wall o f the vessel in which it lives with the ventral sucker. A most distinctive 
feature is the large ventral grove, the gynaecophoric canal, in which the female is retained 
during pairing. The external surface is characterized by an abundance o f  papillae 
(Erasmus, 1987).
Externally, the body is covered by a tegument, which may bear spines, 
tuberculations and/or hairs. The tegument is an acellular, syncitial layer bounded 
externally by a plasma membrane composed o f two bilipid membranes. In vitro studies by 
Sturrock (1993) indicates that the outer bilipid membrane is shed continuously and 
replaced by the products o f  organelles in the deeper syncytium o f the tegument. This 
might presumably happen in vivo. The tegument is a living tissue capable o f taking up 
nutrients and other essential substances, especially inorganic ions (McLaren, 1980). 
Circular and longitudinal muscles below the tegument and other specialized muscles are 
coordinated by a network o f fibres to allow body contractions and other movements. The 
remaining organs are embedded in mesenchymatous cells (Sturrock, 1993).
Waste products are excreted by the two longitudinal canals, which open posteriorly 
and are fed by connecting tubules. There are flame cells whose function is to fan fluid 
wastes into the tubules by means o f  the vibratile cilia with which they are equipped 
(Manson-Bahr and Bell, 1991).
Proteolytic enzymes secreted by cells lining the gut act on host blood ingested 
through the mouth, breaking down serum globulins and haemoglobin from RBC into 
tyrosine (Sturrock, 1993). Schistosomes feed onliquid material in the host in which the 
worm lives and obtain oxygen from the blood ofthe host (Manson-Bahr and Bell, 1991).
The life span o f  the schistosome worm has been the subject o f  controversy. On the
basis o f deita obtained from persons who left an endemic area and who years later were
found to be still passing eggs, a claim has been made that the worm can live up to 30 years
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(Adel, 1990). The mean life span o f  the worm, however seems to be much shorter. 
Warren et al, 1974 reported o f  a study outcome where a group o f Yemeni immigrants 
moved to a non-endemic country, the mean life span of S. mansoni worm was shown to be 
5-10 years. In S. haematobium infections, investigations suggest that its life span may 
even be shorter than that o f S. mansoni (Anderson, 1987).
Schistosomiasis in Ghana
Ghana is among the countries with the highest prevalence rates o f urinary 
schistosomiasis (Berquist, 1987). It is widespread in most parts o f country (Ashitey et al., 
1974). The snails responsible for the transmission o f  the urinary schistosomiasis in Ghana 
are the Bulinus trancatus and B. globosus (Odei, 1961; Onori et al., 1963). B. globosus is 
reported however to be the most important and widely distributed in the country.
The construction o f the Akosombo dam on the Volta River, and the subsequent 
formation o f the Volta Lake altered the existing physical, biological and the socio­
economic environment o f  the people. Although the lake and the head pond created a 
number o f  developmental possibilities in fisheries, transport, agriculture, wildlife and 
tourism, they also created a number o f public health problems, such as the incidence of 
schistosomiasis. The formation o f the lake led to an explosion o f  aquatic weeds to which 
snail vectors o f schistosomiasis attach and feed. In addition, organic materials in the lake 
increased as a result o f the submerged vegetations, providing source o f nutrients for the 
snails. This led to an increase in the population o f  B. truncatus in the lake (Odei, 1973). 
These problems notwithstanding, there was an accompanying increase in fish population. 
This attracted a number o f  fishermen, especially from the area o f the Volta Delta, which 
was highly endemic for schistosomiasis (Kalitsi, 1973). The lake, which is the world’s 
largest artificial lake, has approximately 90% o f the children in the neighboring villages’ 
infected with schistosomes. They often contaminate their environment creating continual 
cycle that leads to poor School performance and growth. Most Africa’s dams are known to
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have similar problems. For instance after the construction o f the Diama Dam on the 
Senegal River in Mauritania, transmission rates rose to new heights. This introduced 
schistosomiasis to both Senegal and Mauritania. Other Dams such as Kainji in Nigeria and 
Kariba in Zimbabwe have contributed to the prevalence and spread o f schistosomiasis.
Today, urinary schistosomiasis has become the main problem associated with the 
Volta Lake. This is accompanied by the fact that the inhabitants depend completely on the 
lake water for their domestic use. There is no proper human waste disposal system and the 
inhabitants freely urinate and defeacate at the lakeshore, perpetuating the cycle of 
schstosomiasis transmission (Kalitsi, 1973). It is reported that villages located closer to the 
lake generally showed a higher schistosomiasis infection rate than those situated further 
away. In a survey o f school children from the village o f Mepe, it was shown that the 
prevalence o f schistosomiasis in children who had never visited the Volta Lake was only 
10.7%, whereas those children who had visited the lakeside at least once had a prevalence 
o f 69.9% (Jones, 1973).
The intestinal form o f schistosomiasis is also known to occur mostly in the northern 
and south-eastern parts o f  the country (Papema, 1968). Though the intermediate snail host 
(Biomphilaria. Pfeifferi) is widely distributed in the entire country most of them are 
however uninfected (Wen, personal communication). The contributions o f other species 
such as S. mekongi and S. intercalatum to human infection are not known. Furthermore, it 
is not documented if any o f the animal schistosomes are present in Ghana. Yet some of 
these animal parasites such as S. bovis occasionally infect humans (Rollinson and 
Southgate, 1987).
Schistosomiasis in Ghana is an important occupational hazard associated with
fishing and fanning. However large numbers o f children and women are also infected as a
result o f  domestic and recreational activities. A stratified random samples o f schools of
the Suhum Kraboa Coaltar District for prevalence and intensity of urinary schistosomiasis
by Ashitey et al, (1974) showed overall prevalence o f 56.9% and that schools with high
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prevalence above 60% were close to the three main rivers, Densu, Suhum and Kua. 
Interestingly, out of 23892 new attendants, only 161 cases o f urinary schistosomiasis were 
recorded in Suhum hospital. In 1994, a prevalence o f 67.7% for urinary schistosomaisis 
and 68,9% for intestinal schistosomiasis in the Kasene-Nankana District in the upper east 
region o f  Ghana was attributed to the Tono Irrigation Scheme. It was also reported by 
Aryeetey et al, (2000), an overall prevalence o f  S. haematobium infection varying between 
54.8 and 60.0% in the Southern Ghana at three defined rural areas drained by the Densu 
River. This indicates that urinary schistosomiasis is a major public health problem in this 
area.
In recent times, both S. mansoni and S haematobium have been reported to spread 
in Ghana and overlap in hyperendermic areas where the schistosomiasis snail hosts coexist. 
This has resulted in mixed infections involving both S. mansoni and S. haemaobium with 
more complicating effects on children. In 1996, an S. mansoni prevalence o f 10.3% and a 
22.5% mixed infection rates were recorded in Sogakope, a town in southeastern Ghana. In 
the same year a urinary Schistosomiasis prevalence o f 47.6% was recorded in Mayera, a 
village in the Greater Accra Region o f Ghana (Bosompem et al., 1996b). Furthermore, 
this disease has severel effects on economic development of the country as it impacts 
negatively on the vast tourist and irrigation potential of the Volta and other Lakes. 
Unfortunately the picture regarding animal schistosomiasis and its effect on human in 
Ghana is yet to be determined.
Animal schistosomiasis
Natural infections o f  domestic and wild animals with human schistosomes have 
been investigated by several workers (Barbosa et al., 1953; Pesigan et al., 1958; Nelson et 
al., 1962; Fenwick, 1969; Mansour, 1973). Nelson, (1960) concluded that all schistosomes 
infecting man in Africa are zoonotic and that the disease is naturally transmitted between
reserviour hosts and man. In some other parts o f  the world (such as China and
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Philippines), where human schistosome infection and disease have been reduced, further 
reduction seemed difficult because o f  the continual transmission from infected animals 
(McGarvey et al., 1998). Natural survey data in China indicated an S. japonicum  
prevalence o f  7% among cattle and 9.6% in water buffalo. Although infection rates o f  10­
15% were found in pigs and in water buffalo, specific community studies in endemic 
Provinces showed higher prevalence rates in cattle. Studies o f the spatial distribution o f 
animal faeces in the lake and marsh regions, and the mountainous regions o f  China 
suggested that cattle dung contributes substantially to potential transmission o f S. 
japonicum  infection (McGarvey et al., 1998).
An epidemiological study o f  S. japonicum  in domestic animals in two 
municipalities o f  the eastern coastal plain o f  Leyte, Philippines, showed that pigs had the 
highest rates o f  prevalence. They found out that dogs had the highest mean 24-hour-egg 
output, and pigs had the highest proportion o f hatchable eggs. However, dogs’ served 
important role in maintaining the transmission o f  the parasite as indicated by a high 
transmission potential and the close habitual contact o f  the animal to humans (Fernandez et 
al., 1982).
In Zambia, schistosomiasis is reported to be endemic with occurrence o f S. 
haematobium and S. mansoni in man and S. matheei, S. margrebowiei and S. leiperi in 
domestic and wild animals. Schistosoma haematobium  and S. metheei are the most widely 
distributed species and their transmission overlaps in rural areas where man and domestic 
animals utilize the same water bodies. It is significant to note that B. globosus is the 
intermediate host for both species (Vercruysse et al., 1994). Similarly in a study in 
Senegal, Albaret et al, (1985), reported that Bulinus umbilicatus is the principal vector of 
S. curassoni (the dominant species in domestic ruminants and in man) and S. haematobium 
(existing in pure infections and in mixed infections with S. curassoni in man)
Studies based on the morphological characteristics o f  eggs in South Africa,
Zimbabwe and Zambia have revealed incidental S. matheei infections in man. Wright,
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Southgate and Ross (1979) demonstrated that S. haematobium and S. matheei readily 
hybridize in man and that FI hybrids are both viable and fertile. Pitchford (1977) therefore 
suggested that in time the two species would be supplanted by a single species, which may 
infect man and cattle with equal ease. Jiang et al, (1997) conducted investigations in 
highly endemic areas o f schistosomiasis japonica in Weishan and Aryans countries. It was 
observed that, the number o f  domestic animals was increasing annually and the proportion 
o f animal husbandry gains in the total agriculture income had a yearly escalating tendency 
and that infection rate o f inhabitants was upgrading as a result o f the development o f 
frequent irrigation o f  domestic animals. Owing to frequent irrigation o f  domestic animals, 
serious spread o f  infection sources and high prevalence o f  schistosomiasis japonica 
occurred.
Van Wyk (1983) reported that in Southern Africa schistosomiasis is practically as 
widely disseminated in animals as in humans. The prevalence in animals is very high in 
certain areas, for instance up to 90% in parts o f the lowveld o f  the Transvaal. S. matheei 
was the only schistosome o f importance in animals in South Africa, with exception o f  S. 
mansoni, which had been recovered from primates and rodents and a single waterbuck 
(Pitchford, 1977) and S. haematobium recovered from one buffalo (Pitchford, 1977). S. 
matheei was discovered in 1926 by Veglia and in 1929 Le Roux (Veglia and Le Roux, 
1929) reported S. matheei in sheep near Humansdorp in the eastern Cape Province and 
recovered S. matheei ova from cattle faeces on the same farm. It shares the intermediate 
snail host, Bulinus (Physopsis) sp. with the human schistosome S. haematobium. Apart 
from South Africa, S. matheei occurs in most neighbouring territories and as far as parts o f  
Tanzania, Chad and Nigeria (Pitchford, 1977). It has the ability to develop in humans as 
cattle schistosome ova have been demonstrated in both urinary and intestinal infections in 
humans in Southern Africa by numerous workers (Alves, 1949; Pitchford, 1959; Cawston, 
1922; Blackie, 1932; Kisner el al., 1953; Cruz, 1971).
In Ghana however, the contributions o f other schistosome species such as S.
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mekangi S. bovis and S. intercalation to human infection is not known. Personal 
communication with researchers at Animal Research Institute and Dr. Wen o f the 
Schistosomiasis Control Unit o f  the Ministry o f  Health, Ghana revealed that currently there 
is no documentation on animal schistosomiasis. Thus the picture regarding animal 
schistosomiasis and its effect on human in Ghana is yet to be determined. Consequently 
veterinary epidemiological studies are urgently needed to improve the understanding o f the 
zoonotic implications o f  the disease and to create a basis for suitable control measures in 
domestic animals if  any.
Schistosome antigens
Attention has been focused on the schistosome surface as a primary source o f  
parasite antigens for protective purposes and as a major site o f immune attack. A variety 
o f  antigens secreted or excreted by the different life stages (adult worm, miracidia hatching 
fluid o f  viable eggs) o f  schistosomes are present in the circulation and/ or the urine o f  the 
infected host (Hermann, 1993). These have different antigenic stimuli. Several o f  the 
schistosome surface antigens have now been identified and a number have been cloned; 
many are glycoprotein, with both the peptide and carbohydrate components acting as 
important epitopes. Some o f these epitopes are shared between different life cycle stages, 
providing a molecular basis for phenomena such as concomitant immunity and generation 
of blocking antibodies. A variety o f  other antigens o f  internal origin are released as the 
worm feeds and metabolizes (Hermann, 1993).
Adult Worm Antigen (AWA)
A detailed analysis by Norden and Strand (1984) of adult worm antigens 
recognized by sera from patients infected with S. mansoni, S. haematobium or S. 
japonicum  concentrated on antigens present in the glycoprotein fraction prepared by 
affinity chromatography using Concanavalin A. This fraction was used based on the
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previous work by Strand et al. (1982) showing that it is the most antigenic. Twenty to 
thirty polypeptides out o f about 50 from each schistosome species were found to be 
antigenic as revealed by immunoprecipitation with the homologous infection sera. Sera 
from S. haematobium precipitated all but 3 o f the antigens recognised by S. mansoni sera 
amongst the glycoproteins. However, a lower degree o f cross reactivity was observed 
using sera from patients infected with S. japonicum.
Kelly et al. (1987) described similar findings by comparing antigens 
immunoprecipitated from cell free translation product synthesized from adult worm 
mRNA o f S. mansoni and S. haematobium. Approximately 40 strongly labelled 
polypeptide antigens were resolved following 2-dimensional polyacrylamide gel 
electrophoresis and immunoprecipitates obtained by using homologous human infection 
sera. Once again extensive cross-reaction was evident with only three S. haematobium 
antigenic polypeptide (Mr 45,000, 27,000 and 14,000) being recognized specifically by S. 
mansoni infection sera.
The significance o f these studies is that they give an indication o f the antigenic 
complexity o f the schistosomes. O f the three major species which infect humans, it 
appears that S mansoni and S. haematobium may be more closely related antigenically to 
each other than to S. japonicum , although a relatively small proportion o f  the polypeptides 
antigens is specific to any one species (Kelly, 1987).
Schistosomula Surface Antigens
A preferred parasitic stage for generation o f monoclonal antibody to schistosome
antigens is the schistosomulum. During the transition from cercariae into schistosomula,
the trilaminate surface membrane o f cercariae matures into a double unit bilayer that
covers the schistosomula (Hockley and Mclaren, 1973). This surface membrane contains
stage-specific glycoproteins, which may represent targets for the host’s immune response
(Hockley and Mclaren,). Monoclonal antibody that recognise surface antigens of
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schistosomula have therefore been sought.
By far, the majority o f studies o f  schistosomulum surface antigens have 
concentrated on S. mansoni. The frequent technique used to identify surface antigens 
include radio-iodination o f  live, freshly transformed schistosomula, followed by the 
immunoprecipitation with a variety o f antisera.
Numerous polypeptides generally o f Mr 100,000 have been labelled using 
lactoperoxidase-catalysed iodination by Ramasay, (1979) and Snary et al. (1980). Dissous 
et al. (1981) also identified a set o f  antigens o f  Mr 32,000-40,000 by precipitation with 
immune rat sera. Schistosomula surface antigens o f  S. haematobium have also been 
identified using iodogen-catalysed labelling followed by immunoprecipitation with human 
infection sera (Simpson et al., 1985). Major antigens o f Mr 17,000 and a complex o f  Mr 
24,000-30,000 have been observed. Similar techniques had been used to identify surface 
antigens o f  S. japonicum.
Most o f  the schistosomulum surface antigens are glycoxylated and both 
carbohydrate and polypeptide moieties contribute to their antigenicity. It is reported that 
surface polypeptide epitopes can induce protection (Kelly, 1987). Polypeptides antigens 
present on the schistosomulum surface are therefore strong candidates as antigens capable 
o f mediating immunity. They are recognised either singly or in combination by 
monoclonal antibodies that passively transfer protection in experimental animals. 
Importantly, they also elicit an antibody response in human patients and do not appear to 
show significant antigenic diversity. A number o f  monoclonal antibodies against the Mr
20,000 antigen have been produced (Tavares et al., 1984; Yi et al., 1986b) and although to 
date, none has consistently transferred immunity, in some experiments statistically 
significant levels o f  protection have however been obtained (Kelly, 1987).
Substantial evidence for the involvement o f surface antigen in immunity is 
provided by the observations that schistosomulum surface antigens o f S. mansoni, S.
haematobium and S. japonicum  show species specificity, whilst the somatic antigens show
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considerable cross reaction (Kelly, 1987). The first immunization studies using purified 
antigens were reported by Smith and Clegg (1985), who used the protective monoclonal 
antibody WP66.4, which recognized schistosomulum surface antigen o f  Mr 200,000 and
38,000 to purify a cross-reacting antigen o f  Mr 155,000 from adult worm. In addition, an 
antigen o f Mr 53,000 was purified from schistosomula extracts using a further MoAb 
which had previously been shown to bind the schistosomulum surface but which was not 
protective.
Schistosome Egg Antigens (SEA)
Many o f the eggs produced by schistosomes do not reach the external environment 
but are swept to the liver by the portal blood flow where they impact on the presinusoidal 
capillaries (Saad et al., 1994). Proteolytic enzymes are considered important mediators in 
the egg migration process from the site o f  ovipositor to the lumen o f the gut or the bladder. 
The mature eggs secrete through the micropore in the eggshell, a complex mixture o f 
antigens that elicit both cellular and antibody-mediated immunologic response (Smither 
and Doenhof£ 1982; Saad et al., 1994).
Soluble egg antigens contain multiple glycoproteins, polysaccharides and non- 
glycoconjugated proteins (Carter and Colley, 1978 and 1979). Warren (1972) reported that 
SEA extracted from the schistosome egg by homogenization and ultra centrifugation could 
trigger o f granulomatous hypersensitivity and other immune reactions typical o f intact 
eggs.
Egg antigens may vary considerably in concentration among schistosome eggs of 
different geographic origin. A major egg glycoprotein was shown to be four times 
abundant in a Puerto Rican strain o f S. mansoni than in an Egyptian strain (Hamburger et 
al., 1982). Also Pelley et al. (1976) noticed intraspecies differences at the protein level by 
comparing protein o f  SEA among S. mansoni strains from different geographical regions
using high performance SDS-polyacrylamide gel capillary electrophoresis.
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Three egg antigens (major serologic antigens- MSA1, MSA2 and MSA3) have 
been purified from S. mansoni (Hamburger et al., 1976 and Pelley et al., 1976) and 
serological studies suggested that only MSA1 (negligible amount in immature eggs, but 
abundant in mature ones) was egg stage and species specific.
Nibbeling et al. (1998) demonstrated that 16 monoclonal antibodies were reactive 
with S. haematobium SEA in addition to S. mansoni SEA. The MoAbs were tested as 
possible immunodiagnostic reagents in homologous sandwich ELISA format to detect 
circulatory SEAs in serum and urine samples o f  S. mansoni or S. haematobium infected 
individuals. In another study, De Brito et al. (1998) reported that adult worm antigen 
(AWA) and SEA were localized ultrastructurally by immunoelution microscopy using two 
MoAbs in the glomeruli o f hamsters infected with S. mansoni cercariae or injected with S. 
mansoni eggs. Both SEA and AWA were present mainly in cytoplasm o f mesangial cells, 
matrix and glomerular basement membrane. Their findings suggested that egg antigens 
contribute to the pathogenesis o f experimental glomerulopathy in the hamster.
Detection o f  circulating SEA is very important in the sense that it may provide 
complementary data to those o f circulating adult worm antigens. This may enable a more 
sensitive level o f antigen detection in a similar way to that found in parallel testing for 
CAA and CCA (Van Lieshout et al., 1991). The measurement o f  SEA levels may also 
provide a more accurate representation o f  tissue egg burdens since it is the eggs that 
produce a great deal o f  the morbidity associated with S. mansoni infection and assessment 
of SEA levels could become a more accurate index o f  morbidity than existing diagnostic 
test. Finally assessment o f  SEA could also be used to measure the effects o f  anti-fecundity 
thereby providing a tool in monitoring effect o f  new vaccines.
Cross- reactive schistosome antigens
There are some egg antigens, which cross-react with other stages o f the parasite.
Von Lichtenberg et al. (1963) showed that mice immunized with eggs developed
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antibodies, which reacted with the cercarial surface. Ham et al. (1984) produced anti-egg 
monoclonal antibodies that bound to the schistosomulum surface. In another study, Yi et 
al (1986a) described four MoAbs, which recognized epitopes present in all stages o f the 
schistosome life cycle. There is enough evidence that much o f the cross-reaction between 
the schistosomulum surface and the egg is due to shared carbohydrate epitopes (Omer-Ali 
et al., 1986). The epitopes, as indicated, are not species-specific and it is thus suggested 
that the stimulation o f antibody recognizing such carbohydrate epitopes may be a factor in 
cross-specific concomitant immunity.
Attallah et al. (1998) reported a polypeptide (Mr 7,000) in antigenic extracts o f the 
three developmental stages (egg, cercaria and adult worm) o f S. mansoni by western 
blotting. This antigen was isolated and purified from crude soluble worm antigen 
preparation by immunoaffinity chromatography using CNBr-activated sepharose-4B beads 
coupled with the BRL4 MoAb.
Excretory-secretory Antigens
Excretory-secretory group o f antigens consists o f  polypeptides, glycoproteins, 
proteoglycans and polysaccharides (Nash and Deelder, 1985; de Jonge, 1990). They are 
gut-associated antigens present in the vomitus and in excretory-secretory materials o f adult 
schistosomes and are released into circulation o f  the host by the regular regurgitation of 
digested blood. These antigens were described by Bergren and Weller (1967) as 
circulatory by virtue o f  the fact that they are found constantly in the blood and other body 
fluids o f infected individuals. Their presence in a patient therefore indicates an active 
infection with viable worms (Hermann, 1993).
Two proteoglycan gut-associated antigens (circulating anodic and circulating 
cathodic antigens, CAA, CCA) have been detected in serum, urine and breast milk o f 
African and South American patients with schistosomiasis mansoni (Santoro et al., 1980;
Feldmeier et al., 1986b; de Jonge et al 1990) in serum and urine o f  patients infected with
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S. haematobium or S. intercalatum (Feldmeier et al., 1986b; de Jonge et al., 1989b) and in 
serum o f Filipinos infected with S. japonicum  (Vant Wout et al., 1992). This supports the 
report by Bawden and Weller (1974) that the CAA was not species-specific by 
demonstrating its presence in S. mansoni, S. haematobium  and S. japonicum  adult worm 
homogenates and in the sera o f  mice and hamsters heavily infected with either S. mansoni 
or S. japonicum. CAA as described by Gold, Rosen and Weller (1969) are heat stable, 
dialyzable and anodic as determined by its immunoelectrophoretic mobility unlike the low 
molecular weight CCA, which is cathodic.
Other circulatory antigens have also been identified and characterized. Crabtree 
and Senft (1974) described several purine salvage enzymes (adenosine phosphorylase, 
adenosine kinase, adenosine deaminase and purine nucleotide phosphorylase) present in 
schistosome vomitus (excretory-secretory gut product). These enzymes could incite 
histaminic skin reactions (reagenic responses) in the host.
Enzyme-linked Immunosorbent Assay (ELISA)
One o f the most widely used applications o f MoAbs is enzyme-linked 
immunosorbent assay (ELISA). ELISA is based on antibody recognition o f a particular 
antigenic epitope. It combines the specificity of antibodies with the sensitivity o f simple 
spectrophotometric enzyme assays by using antibodies or antigens coupled to an easily 
assayed enzyme that also possesses a high turnover number (Wilson and Walker, 1995).
ELISA is replacing radioimmunoassays because o f the lack o f  radio hazards. It is 
also extremely economical in the use o f reagents (Riott et al., 1993); large numbers o f  tests 
can be performed in a relatively short time. Also the enzyme conjugates are more stable 
than radioactive isotypes (McMichael and Beverley, 1986).
For screening, an indirect method is invariably used in which an appropriate 
enzyme is covalently coupled to anti-mouse or rat immunoglobulin antibody (McMichael 
and Beverley, 1986). Binding enzymes are selected which show simple kinetics and can
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be assayed by a simple procedure (normally spectrophotometric). The most commonly 
used enzymes are the alkaline phosphatase, B-D-galactosidase and horseradish peroxidase. 
Binding o f anti-immunoglobulin is detected by conversion o f enzyme substrate to a 
coloured reaction product or precipitate.
The putative antiserum is reacted with specific antigen attached to a solid phase. 
Solid phases commonly used in ELISA include cross-linked dextran or polyacrylamide 
beads, filter paper (cellulose) discs (membrane-based ELISAs) and disposable polystyrene 
microtitre plates (plate ELISAs), which are convenient for large numbers o f samples. The 
appropriate antigen or antibody may be attached to the solid phase by passive adsorption or 
covalent coupling with cyanogen bromide.
Colourless substrates that are converted to a coloured product by the enzyme are 
popular. For instance, p-nitrophenylphosphate (pNPP) is converted to the yellow p- 
nitrophenol by alkaline phosphatase. Substrates used with peroxidase include 2,2-azo-bis 
3-ethylbenzthiazoline-6-sulphonic acids (ABTS), O-phenylenediamine (OPD), and 3,3’, 
5,5’-tetramethylbenzidine base (TMB), diaminobenzidine tetrahydrochloride (DAB), yield 
green, orange, blue and brown colours respectively. In all ELISAs reference positive and 
negative samples must be included in each series o f  tests to ensure accurate and 
reproducible results.
ELISA can be used for the assay o f  virtually any antigen, hapten or antibody. It is 
used predominantly in clinical biochemistry in the study o f infectious diseases including 
detection o f bacterial toxins. It is also used to assay antibodies in infectious diseases 
including Plasmodium, Schistosoma and Trypanosoma spp.
Monoclonal Antibodies (MoAbs)
Antibodies or immunoglobulins (Ig) are a group o f  glycoproteins present in the 
blood serum and tissue fluids produced by B-lymphocytes. They are the soluble form o f 
the B cells antigen receptor. All antibodies have the same basic structure but they are
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diverse in the region that binds to the antigenic determinant site (epitope) o f  the antigen. 
The epitopes may be either peptide or carbohydrate in nature or more rarely lipid. One 
part (Fab) binds to antigen and the other parts (Fc) interact with other elements o f  the 
immune system. Antibodies allow the immune system to recognize specific pathogens and 
their products (Roitt et al., 1993).
Many different antibodies (polyclonal antibodies) secreted against several antigen 
epitopes are found in the immune sera. As a result immune sera are non-specific to any 
one particular determinant and cross-react with antigens from various sources (Campbell, 
1984). They are therefore not suitable for assays in which antibody specificity is crucial. 
Polyclonal antibodies are particularly valuable for immunoprecipitation and 
immunoblotting. Prior to 1975, it was possible to only produce polyclonal antibodies. 
Kohler and Milstein (1975) developed a procedure to produce monoclonal antibodies from 
hybridoma cells. These are cells formed by fusion o f B-lymphocytes (antibody producing 
cells) from the spleen o f  an immunized animal, with a myloma cell that has the capacity 
for unlimited proliferation (immortal). The single fused cell possesses the property o f  the 
immortal cell and the specific antibody production. The hybridoma can then be injected 
into animals to induce antibody-secreting myloma cells to produce antibodies collected in 
ascites (in vivo) or they can be grown in mass culture to produce specific antibodies (in 
vitro).
Antibodies produced by monoclonal hybridomas have many outstanding 
advantages over the conventional antisera. Apart from their monospecificity, specific 
antibody is available in concentrations several orders o f  magnitude greater than in the 
conventional sera and can be derived for almost any purpose. It is possible to introduce 
stable internal labels into the antibody molecule by culturing the hybridoma cells with 
radiolabelled amino acid, a possibility not available with the conventional sera 
(Rosemarine, 1986). These advantages have made certain experimental techniques much
simpler and more reliable and perhaps more importantly, have allowed the development of
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powerful experimental approaches not possible with conventional antibodies.
Uses o f  Antibodies
Monoclonal antibodies are in effect homogeneous immunological reagents o f 
defined specificity, high specific activity and selected isotype. They have been established 
as exceptionally powerful research agents and also with potential clinical uses. In 
immunochemistry, MoAbs have been utilized for determining the structure and 
biochemical characteristics o f  molecules. They have made possible monospecific reagents 
o f  veiy high specific activity to virtually any molecule o f  interest, bringing the possibility 
o f  using immunochemical techniques to almost every laboratory. Monoclonal antibody 
techniques have provided an opportunity to re-evaluate the role o f  immunological methods 
for the diagnosis o f infectious diseases. Antibodies o f diagnostic potential have therefore 
been prepared in research laboratories against a battery o f viruses, bacteria fungi and 
parasites (Nowinski et al., 1983).
In a study by Nowinski et al, (1983) the diagnostic utility o f  monoclonal antibodies 
for gonococcal, chlamydial and herpes virus infections were described. The antibodies 
used demonstrated sensitivity o f 94-99% for culture confirmation and 85-90% for direct 
diagnosis o f specimens smeared on microscope slides. They have significant impart on the 
characterization o f parasite antigens in schistosomiasis (Ham et al., 1985; Capron et al.,
1987). Advances toward antigen analysis using MoAbs are o f  particular importance in 
defining relevant antigens to be selected for possible vaccine development (Simpson and 
Coli, 1987).
Purification o f  Antibodies
Purification and characterization is a prerequisite to studying biological molecules. 
Purified antibodies are requires for a number o f techniques.
MoAbs produced in culture supernatants and ascites may contain impurities that
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can ultimately affect the reactivity and or the sensitivity o f the antibody. Particularly, 
antibodies present in the form o f ascites are generally not ideal for use without some form 
o f purification to remove contaminants such as the oily solutions used to induce and 
promote ascites formation. Also the common media used for the growth o f  MoAb- 
producing cells in vitro and supplements with fetal bovine serum (FBS) or fetal calf serum 
(FCS), which may account for about 10% o f the complete medium. These serum 
supplements (proteins) usually serve as contaminants and they interfere in some o f the 
assays that utilize MoAbs. Notwithstanding, unpurified antibodies can be perfectly used in 
cytotoxicity studies if the concentration o f the antibodies is not important.
There is a wide variety o f  methods to purify antibodies and the correct choice of 
purification will depend on a number o f factors including (1) the manner in which the 
antibody will be used (2) the species in which the antibody was produced (3) the class and 
subclass and (4) the source (ascites or tissue culture supernatant).
The most commonly used method in the purification is ammonium sulphate 
precipitation. The concentration at which antibody is precipitated varies from species to 
species but most antibodies will precipitate at 50% saturation. A disadvantage o f the 
ammonium sulphate method is that the resulting antibody will not be pure. They will be 
contaminated with other high molecular weight proteins, as well as proteins that are 
trapped in the large flocculant’s precipitate. Therefore ammonium sulphate precipitation is 
not suitable for single step purification but must be combined with other methods if a pure 
antibody is needed. The antibody isotype is one o f  the most important factors that 
influence the choice o f protocol for subsequent purification (Goding, 1986). For instance, 
IgG monoclonal antibodies are best purified by ion-exchange chromatography whilst IgM 
antibodies require gel filtration.
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Diagnosis of human schistosomiasis
The control o f  schistosomiasis is an urgent task, which requires unproved diagnosis 
and treatment as well as effective prevention (Han Xu et al., 1989). Decisions on 
prognosis and assessment o f  morbidity, evaluation o f chemotherapy and control measures 
all build on the results from diagnostic tests (Hermann, 1993). It is thus important to select 
a diagnostic tool that corresponds to the type o f information sought by the clinician or the 
epidemiologist. There is therefore the need for more simple, rapid, sensitive, reproducible 
and cost effective diagnostic test for schistosomiasis.
There are three different approaches for the diagnosis o f the disease. These are the 
(1) direct parasitological methods, which detect schistosome ova in urine, stool or the 
rectal mucosa and histological methods disclose schistosomula, adult worm or eggs in 
tissue biopsies, (2) indirect methods which rely on clinical, biochemical or immunological 
disease markers, detect pathology typically or frequently associated with schistosome 
infections and (3) immunological methods which measure the immune response to certain 
schistosome antigens or the concentration o f  parasite-derived antigens in blood or urine 
(Hermann, 1993).
Eggs in urine
The intensity o f  schistosome infection is measured by quantitative egg counts, 
which are highly variable (Deelder et al., 1989) and may depend on the immune status o f 
the host (Damian, 1987).
Urine samples may be examined under microscope for S. haematobium eggs. This
method has been widely used in individuals and community diagnosis (WHO 1983c). The
method is simple, rapid, specific but not very sensitive. The sensitivity can however be
increased if (1) samples are collected at noon where egg secretion is maximum, (2)
examination o f the sediment from large volume o f urine (Peters and Kazura, 1987). It is
generally accepted that the excretion of eggs in urine follows a circadian rhythm with a
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peak around noon. Since eggs are responsible for the presence of lower renal track 
pathology in schistosomiasis haematobium, measurement o f  haematuria, proteinuria and 
leucocyturia also varies with the time o f the day (Doehring et al 1985a, b).
Urine sediments may be obtained by centrifugation or filtration. In filtration, 
paper, polycarbonate, polyamide or membranes derived from other synthetic fibres may be 
used. The membranes differ in properties (Bradley, 1965; Peters et al., 1976; Pugh, 1978). 
Paper filters have to be stained in order to allow identification o f schistosome ova. On 
polycarbonate membranes, ova are more easily identified (Hermann, 1993). Staining with 
1.0% trypanblue facilitates visualization and allows discrimination between viable and 
non-viable ova (Feldmeier et al., 1979). Other stains in use include 5-10% tincture of 
iodine or solutions o f eosin, methylene blue or ninhydrine.
Centrifugation is a valuable alternative to filtration. Richards et al, (1984) 
emphasized that the sensitivity o f centrifugation compares favourably to that o f the usual 
filtration o f  10ml in low intensity infection.
It is worth noting that egg detection in urine has drawbacks. It may be biased in 
urine o f females o f childbearing age. This is because the epithelial cells frequently in 
female urine tend to clog filter membranes, which may completely disguise schistosome 
eggs. Also when urine is contaminated with menstrual blood, lysis o f  erythrocytes is 
required to disclose ova in sediments or on filter membranes. This may usually be 
achieved by addition o f  10% HC1 to urine sample (Feldmeier et al., 1979).
Eggs in Stool
The ideal field method for the detection o f  schistosome ova in stool is still lacking 
(Hermann, 1993). Currently, the technique described by Kato and Miura (1954) for 
diagnosing hookworm/Ascaris infections, which was amended by Katz et al. (1972) and 
modified by several workers (Teesdale and Amin, 1976; Peters et al., 1980) has been 
widely accepted as a valuable compromise for fieldwork. A specified amount o f  stool
specimen cast by a template is treated with 50% (v/v) glycerol in water containing 3%
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malachite green before microscopic examination. The method is sensitive for the detection 
o f light infection, quick and suitable for large epidemiological studies.
Biopsies
Infections with all human schistosomes can be diagnosed by microscopic 
examination of minute biopsies of the rectal mucosa. Snips are taken from suspicious 
lesion or from the plica transversalis recti. The efficiency o f rectal biopsy has been shown 
in schistosomiasis mansoni (da Cunha, 1982), schistosomiasis intercalatum (Feldmeier et 
al., 1981a) the oriental schistosomes (Maunouiy et al., 1990). Even in infection with S. 
haematobium, eggs are frequently detected in rectal snips (Badran et al., 1955; Harries et 
al., 1986). The biopsies are crushed between two thick cover slips and the surface 
examined. Quantitative results are obtained that significantly correlate to the number per 
gram o f faeces. If few drops o f  glycerol-malachite solution are added to the biopsy before 
compression, viable and non-viable eggs are easily differentiated by morphological aspects 
(Cancado et al., 1965). Rectal biopsies are especially meaningful in the assessment o f cure 
rates after chemotherapy. However, the histological sectioning is invasive and therefore 
limited in application.
Immunodiagnosis
Schistosomiasis remains a serious worldwide public health problem with a still 
unfulfilled need for routine cost- effective method o f diagnosis. Such methods are 
required not only for people in endemic areas but increasingly for tourists who may be 
infected during visits to such places.
The routine parasitological diagnosis o f  schistosomiasis though very specific, is 
beset with a number o f limitations making its use unreliable. These limitations include the 
relative insensitivity in the detection o f low intensity infectious patients; difficulty in 
achieving homogenous distribution o f S. haematobium ova in urine (Braun-Munzinger and
Southgate, 1992) as well as the day-day and circadian variation in egg excretion. This may
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lead to incorrect estimates in prevalence and intensity o f infection (Gryseels, 1994). It is 
also laborious, not field applicable and expensive.
There is therefore the need for differential diagnosis. This must be simple, rapid, 
sensitive, reproducible and cost-effective. The increasing demands for simple and reliable 
assays have been noted in field monitoring o f schistosomiasis in the endemic areas where 
control measures have been taken for years (Qian-Li et al., 1993). It is therefore suggested 
that due to the relative insensitivity o f  both the parasitological and antigen detection, 
antibody detection method could find increasingly use in situations o f  low infection 
intensity (Hamilton et al., 1998).
Numerous schistosome serodiagnostic assays (based on the detection o f host 
antibodies directed against schistosome antigen) with high sensitivity and specificity have 
been developed (Mott and Dixon, 1982; Qian-Li et al., 1993). Detection o f  specific 
antibodies is a valuable tool for immunoepidemiological studies, but antibody levels are, in 
general, not related with the intensity o f  the infection nor are they indicative o f a still 
active infection (Deelder et al., 1994). This does not discriminate between previous 
exposure and current infection (Simpson and Smithers, 1985). Assays that could measure 
circulatory antigens secreted by live parasites and discriminate infections based on their 
intensity might be able to evaluate the efficacy o f  chemotherapy and the effectiveness o f 
future vaccines (Barsoum et al., 1991). All these attributes would be highly desirable. 
Therefore the detection o f  circulatory antigens in schistosomiasis is increasingly used as a 
diagnostic tool, because level o f  antigens is correlated with worm burden and antigen 
would disappear relatively rapidly from circulation after successful chemotherapy (Deelder 
etal., 1994).
Although circulatory antigens may be produced by several life cycle stages, 
including eggs, the most important diagnostic antigens are the CAA and CCA, which are 
associated with the syncytium lining the gut o f  the adult worm (Deelder et al., 1976). The
CAA level in relation to intensity o f infection has been studied in S. mansoni, S.
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haematobium, S. japonicum  and S. intercalatum infections (Deelder et al., 1989; Deelder et 
al., 1990; De Jonge et al., 1988). It was reported that, in general, CAA levels correlated 
with the intensity o f infection as determined by egg output. When CAA or CCA is 
measured quantitatively, antigen concentration in serum or urine significantly correlated to 
the number o f eggs excreted in stool or urine (Santoro et al., 1980; Feldmeier et al., 1986b; 
de Jonge et al., 1989b; Von’t Wout et al., 1992). These findings confirmed the notion that 
the concentration o f gut-associated antigens in blood or in urine is directly linked to the 
number o f adult worm present in mesenteric or prevesical plexus, which in turn determines 
the number o f  eggs passed into the intestine or the bladder respectively.
Following chemotherapy however, CAA levels in serum were found to decline 
rapidly with a half-life o f  2.5 days (De Jonge et al., 1989). Deelder et al, 1994 reported 
similar findings that in S. haematobium and S. japonicum  infections, CCA and/or CAA 
serum levels decreased soon after treatment.
The introduction o f  ELISA and radioimmunoassays has led to improvement in the 
sensitivity o f serodiagnostic techniques for schistosomiasis (Smither and Doenhoff, 1982). 
ELISA however is the preferred option, in that the assay is based on stable antigen- 
antibody complexes and does not require the use o f  harmful radioactive substances.
In a cross-sectional survey, Al-Sherbiny et al. (1999) used serum, urine and stool 
samples from patients in an area known to be endemic for S. haematobium in Egypt. 
Diagnosis was approached in two parallel ways; the physical examination o f urine and 
stool microscopic analysis and two advanced immunodiagnostic assay systems, Falcon 
assay screening test (FAST)-ELISA and the enzyme-linked immuno electro transfer blot 
(EITB). Parasitologically, the overall prevalence o f  S. haematobium was 15.8%. The 
combination o f urine CCA and serum CAA for detecting circulatory antigens and the 
combination of the S. haematobium adult worm microsomal antigens (HAMA) FAST- 
ELISA and HAMA EITB for detecting antibodies significantly improved the sensitivity o f
detecting S. haematobium circulatory antigens and antibodies.
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Diagnosis of animal schistosomiasis
Diagnosis o f animal schistosomiasis is mainly based on the clinico-pathological symptoms 
o f diarrhoea, wasting and anaemia. The relatively persistent diarrhoea, often blood stained 
and containing mucus may help to differentiate this syndrome from faciolosis (Urquhart et 
al., 1988). The routine method o f diagnosis is the microscopical examination for parasite 
eggs in faecal samples. However the demonstration o f  the characteristic eggs in the faeces 
or in squash preparations o f blood and mucus from the faeces is useful in the period 
following high infection but less useful as egg production drops in the later stages of 
infection. Generally when schistosomiasis is suspected, diagnosis is best confirmed by a 
detailed post-mortem examination which will reveal the lesion and if the mesentery is 
stretched, the presence o f  numerous schistosomes in the veins (Urquhart et al., 1988). 
These methods are time consuming and there is therefore the need for alternative diagnosis 
such as serological diagnosis particularly in epidemiological surveys.
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CHAPTER 2
GENERAL MATERIALS AND METHODS
Study area
Two villages, Galilea and Agbekpotsepko, were chosen as study areas based upon 
epidemiological data on the distribution o f schistosomiasis. Galilea is a village in the Ga 
District o f the Greater Accra region. It is located along the Weija Dam, which serves as 
the main source o f  domestic water for the community. The weedy bank o f the dam 
contains large amount o f decomposing plants and twigs and is infested with Bulinus and 
Biomphilaria snails. The dam constitutes a principal source o f  water and transmission o f 
schistosomiasis.
Agbekpotsepko is located in the Dangbe West District o f  the Greater Accra region. 
The vegetation is mainly o f  grass with few trees. The area is swampy and constitutes a 
suitable breeding site for schistosome intermediate snail host. The main occupation o f  the 
community is farming and free range cattle rearing. The sources of water for the 
community are streams, which also serve the cattle. It was therefore suitable to select the 
area to investigate the prevalence o f  animal schistosomiasis.
Resuscitation of Hybridoma Cells
Monoclonal antibody secreting hybridama cell lines cryopreserved in 7.5% 
dimethylsulfoxide (DMSO) in Iscove’s Modified Dulbecco’s Medium (IMDM) were 
retrieved from liquid nitrogen at -196°C. The content o f a vial was thawed rapidly in a 
water bath at 37°C and immediately transferred into a 15ml centrifuge tube containing 
10ml o f sterile growth medium [IMDM supplemented with 10% (v/v) heat inactivated 
(56°C/30min) Foetal Calf Albumin (FCS)]. This was gently mixed and washed by 
centrifugation at 415Xg for 15 min at 37°C to remove the DMSO. The supernatant was
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discarded and the cell pellet resuspended in 3ml fresh growth medium. Approximately 
lm l of cell suspension was transferred into 48 well plates and incubated at 37°C in a 
carbon (IV) oxide (CO2) incubator (MCO 175, Sanyo Japan) at 5% CO2 concentration. 
The moabs produced were Sh3/34.10, Sh3/38.2, Sh4/14.3, Sh5/32.30 and Sh5/34.10
Cloning and Propagation of Hybridoma Cells
Resuscitated hybridoma cells in culture were cloned to ensure monoclonality and 
continuous secretion o f monoclonal antibodies. The cells in suspension were diluted with 
growth medium containing trypanblue (counter stain) to give 0.1% final concentration of 
the stain. Ten microlitres o f the stained cell suspension was dispensed into a Neubauer 
counting chamber and the life cells counted microscopically (X I00 magnification) using 
an inverted microscope (Olympus, Tokyo, Japan). The cells were cloned by limiting 
dilution in growth medium to give 1 cell/ 50 nl/ wellin 96 well tissue culture plates. These 
were cultured at 37°C in a CO2 incubator and left undisturbed for 10 days. The plates were 
then examined for viable cell colonies by viewing the bottom o f the wells or by observing 
under an inverted microscope. Wells with single viable cell colonies were marked and the 
cells transferred into 0.5ml o f  growth medium in 24 well tissue culture plate. After 
incubation for 3 days, 200|il o f culture supernatant from each well was examined for 
antibody activity by micro-plate ELISA. The cells in antibody positive wells were 
transferred into 25cm2 tissue culture flasks and added fresh growth medium for expansion.
The cells were sub cultured by transferring up to 2ml o f the cell suspension into 
larger flasks (75cm2 and 125cm2) and the MoAb containing medium harvested when it 
became acidic (yellowish). Fresh growth medium was added and more antibody 
containing culture supernatant harvested from time to time. The supernatants were 
centrifuged at 415Xg for 5min to remove cell debris and stored at -20°C.
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Cryopreservation of Hybridoma Cells
Cloned MoAb secreting hybridoma cells in logarithmic phase o f  growth were 
centrifuged at 400Xg for 5min. The pelleted cells were resuspended in stabilating medium 
containing 7.5% (v/v) DMSO (E. MERK, Darmstadt, Germany) to make a 2x106 cells/ ml 
suspension. One millilitre aliqouts o f the cell preparation were pipetted into 
cryopreservation vials before freezing in liquid nitrogen using a cryo-controller version 
2.01 (Dept, o f Biomedical Engineering, University Hospital, Copenhapen, Denmark) 
programmed to freeze cells over a period o f 1 hr during which time specimen were 
subjected to a temperature gradient from room temperature to -140°C. The frozen vials 
were removed and immediately transferred onto labelled stabilation rack and immersed in 
liquid nitrogen at - 1 96°C.
Determination of Immunoglobulin Class and Subclass
The MoAb class and subclass were determined using the double Immunodiffusion 
method described by Ouchterlony (1967). Commercially prepared antisera against murine 
Immunoglobulin isotypes IgGl, IgG2a, IgG2b IgG3, IgGM were used. The Quchterlony 
plates were made using 1% (w/v) agarose gel prepared by melting solid agarose in 
phosphate-buffered saline (15mM NaCl, 1.1 mM NaHP0 4  and 0.1 mM KH2PO4, pH 7.4). 
Five millilitres o f the molten agarose was gently poured onto a microscope slide and 
allowed to solidify. Five wells equally spaced were cut into the solid gel in a circular 
arrangement surrounding a central well. Each well could hold approximately 15 (il o f 
reagent. Antiserum was placed in central well and culture supernatants, concentrated thirty 
fold by amicon filtration placed in the surrounding wells. The prepared slides were left in 
a moist chamber overnight and the developed precipitin lines were observed by viewing 
the gels against light. The slides were then pressed under a pile o f  filter papers to dry the 
gel, which was then stained with coomasie blue and photographed.
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Purification of Monoclonal Antiboddies
Monoclonal antibodies in culture supernatants were first concentrated by Amicon 
filtration, followed by ammonium sulphate precipitation and further purified by gel 
filtration.
Amicon Filtration
MoAb containing culture supernatants stored at —20°C were retrieved and thawed at 
37°C in a water bath. Pooled culture supernatant was transferred into an Amicon filtration 
chamber (Nucleopone U.S.A) fitted with 100,000 molecular weight cut-off ultra-filtration 
disk membrane (Sigma, U.S.A). The culture supernatant was concentrated forty-fold by 
filtration under pressure using Nitrogen gas. Concentrated MoAbs were transferred into 
storage vials and either stored at -20°C or purified.
Ammonium Sulphate Preci ~-tation
Monoclonal antibodies in Amicon concentrated culture supernatant were 
precipitated by the slow addition o f saturated ammonium sulphate solution while mixing. 
Ammonium sulphate was added to a final concentration o f 50% (v/v) for IgG and 30% 
(v/v) for IgM. The precipitate formed was pelleted by centrifugation at 1200Xg for 30min 
at 4°C and dissolved in minimum amount of distilled water. The antibody solutions were 
transferred into 1000MW cut-off dialysis membrane bags (Spectro Medical Industries 
Incorporated USA) and dialysed over night on ice against phosphate buffered saline (9mM 
NaH2P04, 0.9mM Na2HPC>4 , 15mM NaCl, pH 7.4) with three buffer changes to remove 
the excess salt.
Gel Filtration
Ammonium sulphate precipitated and dialysed IgM MoAbs were further purified 
by gel filtration on Sephadex G-200 (Pharmacisa, Uppsala, Sweden), pore size 40-120 |itn. 
This was prepared according to the manufacturer s instructions. The gel was allowed to
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swell for 5 hours at 100°C and degassed for 2 hours. A 2.6 x 100cm column was packed 
and washed with at least one column volume o f elution buffer (PBS, 0.138M NaCl; 2.8mM 
KC1; 10.2mM Na2HP04; 1.8mM KH2P04, pH 7.4). Twenty millilitres o f dialysed MoAb 
diluted to reduce viscosity was applied onto the column and eluted with PBS, at a flow rate 
o f 40ml/ hour. The eluates were collected 5ml/ tube and assayed for antibody activity by 
microplate-based ELISA. Fractions containing antibodies were pooled, concentrated by 
Am icon filtration and stored at -20°C until needed.
Micro-Plate ELISA
Micro-plate ELISA was used for detection o f  MoAb in fractionated reagents and in
culture supernatant. Polysterene microplates (Sumilon S type MS-8496F) were coated
with either S. haematobium soluble egg antigen (SEA) or P2J (S. haematobium urinaiy
antigen) at 37°C overnight to dry. The P2J antigen stock was obtained from the
Parasitology Unit o f the NMIMR and the SEA (from an Egyptian strain o f  S.
haematobium) was donated by the WHO. Soluble egg antigen was coated at 1 .O^g/well
and P2J at 0.5(ig/well in carbonate coating buffer. The plates were rinsed once with
washing buffer, PBS pH 7.4, consisting o f  0.136M NaCl, 9.7mM Na2HP0 4 , 1.4mM
KHPO4, 2.7mM KC1, 0.6mM CyHsOzNa and 0.5% (v/v) Tween 80. They were then
incubated with different fractions o f  prepared MoAbs in duplicate wells for 15min.
Undiluted normal culture medium and infected mouse serum diluted at 1:100 were added
as negative and positive controls, respectively. The plates were flipped empty and rinsed
twice with washing buffer to remove excess unbound MoAbs. The wells were then
incubated for 30min (50|il/ well) with either goat anti-mouse IgM horseradish peroxidase
(HRPO) conjugate for detection o f  IgM MoAbs (Sh3/34.10, Sh3/38.2, Sh5/32.30 and
Sh5/34.10) or goat anti-mouse IgG-HRPO for Sh4/14.3. The conjugates were each diluted
at 1:500 in blocking buffer (0.5% BSA in washing buffer). The plates were emptied,
rinsed again and washed further by flooding three times, each with lOmin incubation to
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remove unbound conjugates. The presence o f the bound conjugate was revealed by the 
incubation o f substrate solution (100|j.l/ well) in the dark for 30min. The substrate solution 
[40mM 2,2’azino-bis-3-ethylbenzethiozaline-6-sulphonic acid (ABTS) and 0.01% (v/v) 
H2O2 in 50mM citrate buffer, pH 4.0] changed to green in wells with bound enzyme 
conjugates. Optical densities were read at 415nm wavelength using an MTP-32 microplate 
reader (Corona Electric, Japan).
Cross-reactivity testing of MoAbs using schistosome and P. falciparum  antigens in 
microplate ELISA
The micro-plate ELISA procedure described above was also used to test the 
selected MoAbs for cross-reactivity using antigens o f Schistosoma species (S. 
haematobium, S  mansoni and S. japonicum), and P falciparum  circum-sporozoite protein 
(CSP) and crude antigen extracts obtained from the Immunology Unit o f  the NMIMR. 
Briefly, polystyrene microplates were coated separately with the different antigens 
50|i 1/well at 37°C overnight to dry. The plates were rinsed once with PBS washing buffer 
and incubated 50fil/well for 15min with test MoAbs, starting from neat, 1:5 and then 
diluted up to 1:3200. The plates were rinsed twice with washing buffer and then incubated 
for 30min with 50jil/well o f  goat anti-mouse IgM or IgG conjugate. The plates were again 
washed before incubation with substrate solution.
Preparation of Horseradish Peroxidase Antibody Conjugates
Purified Schistosoma genus-specific MoAbs were conjugated to HRPO using the
periodate method described by Wilson and Nakane (1978). The protein concentration of
antibody fractions was estimated by Buiret Protein assay and HRPO enzyme (Sigma USA)
conjugated to antibody protein at a ratio o f 1:1 (enzyme:antibody) by molecular weight.
Calculated enzyme was dissolved in 2ml o f  50mM sodium acetate buffer, pH 4.0 and
activated (oxidized) using sodium metaperiodate (NalO.*) in the ratio o f 1:1 by weight.
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The required quantity o f NaIC>4 was dissolved in 1ml o f  sodium-acetate buffer, and the 
NaIC>4 solution then added dropwise to the HRPO solution. The mixture was kept in the 
dark for 20min and 300|il ethylene glycol (C2H6O2) added and stirred. The resulting 
mixture was fractionated through a sephadex G-25 column (1 .Ocm diameter x 30.0cm) and 
eluted with sodium-acetate buffer. The pH o f the eluted enzyme and the antibody solution 
were adjusted to 9.6 by the addition o f  l-2ml carbonate-bicarbonate buffer, pH 9.6 
followed by dropwise addition o f saturated Na2CC>3 . The antibody and enzyme solutions 
were then added together, covered with aluminium foil and stirred slowly for lh r at room 
temperature. Three hundred milligrams o f glycine (NH2 .CH2 .COOH) was then added, 
mixed and the pH adjusted to 8.0 using 1M HC1. The conjugate was kept at 4°C overnight, 
after which it was precipitated with 50% (v/v) saturated ammonium sulphate solution and 
then centrifuged for 2 min at 9,900 xg. The pellet was dissolved and made up to the 
original volume with glycine/Na2EDTA buffer (0.4M glycine, 0.3M NaCl and 20mM 
Na2EDTA, pH 8.0). Twenty milligramms o f ovalbumin was added and mixed to dissolve, 
and the solution centrifuged once more to remove particulate matter. The conjugate 
solution was then passed through a 0.45|im, followed by a 0.22|im membrane filter 
(Millipore Products Division, Bedford, MA, USA) to remove polymerised conjugate. 
Finally an equal volume o f glycerol was added, mixed and the reagent stored at -20°C 
until used.
Coating of the Test MoAbs on PVDF and Nitrocellulose Membranes by Dot-ELISA
The ability o f  the test MoAbs to coat onto PVDF membrane (Millipore
Corporation, Bedford MA) and Nitrocellulose membrane (Sigma Chemical Co. USA) was
assessed using PBS o f different pH (7.0, 7.2 and 7.4). Each o f  the MoAbs was diluted
separately in the three different PBS buffers and two microlitres volumes dotted on
membrane strips measuring 1x6cm. PVDF membrane strips were first soaked with
methanol, quickly immersed in distilled water and then placed on moist filter paper before
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dotting the samples. Nitrocellulose membranes were used without prior processing. The 
strips were then air dried for 5 min and incubated in blocking solution (0.3% w/v casein) 
for 30 min with gentle shaking. To assess binding o f MoAb to the membranes, the strips 
were incubated for 1 hr in goat anti-mouse HRPO IgM or IgG depending on the isotype o f 
the test MoAb. After incubation the strips were washed three times (10 min/wash) in 
washing buffer (0.1% Triton X-100 in PBS). This was followed by a lmin incubation in 
substrate solution (25ml TBS, pH 7.4; 0.005g DAB; 150|il cabaltous nitrite; 15pl H2O2), 
and extensive washing in excess distilled water. Positive reactions which, appeared bluish 
black were visually assessed and graded.
Coating of the Selected MoAbs to Micro-titre Plates
Coating o f  the test MoAbs to micro-titre plates was investigated using different 
polystyrene plates; Sumilon (Ms-8496F), Sero-wel (Cat. Cat No. 612F96) and Sero-wel 
(Cat. No. 611U96). Dulbecco’s PBS (pH 7.4) was used as coating buffer. Fifty 
microlitres o f  each dilution o f test MoAb (1:25 —1:3200) was dispensed into wells o f  micro 
titre plates and incubated for 30 min. The plates were flipped empty and washed twice 
with washing buffer [PBS, 0.136M NaCl, 9.7mM Na2HPC>4, 1.4mM KHPO4 , 2.7mM KC1, 
0.6mM CyHsChNa and 0.5% (v/v) Tween 80, pH 7.4] to remove unbound MoAbs. They 
were then incubated for 30 min (50nl/ well) with goat anti-mouse IgM-HRPO conjugate or 
goat anti-mouse IgG-HRPO diluted at 1:500 in blocking solution (0.5% Bovine serum 
albumin in washing buffer). After incubation, wells were washed further by flooding three 
times (lOmin/wash) to remove unbound conjugates. The presence o f  the bound conjugate 
was revealed by the addition o f ABTS substrate solution (lOOpl/well) for 30min in the 
dark and the optical densities read at 415nm wavelength using an MTP-32 microplate 
reader (Corona Electric, Japan).
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Dipstick ELISA procedure
Polyvinylidene difluoride membrane was cut into strips o f  dimension 2mm by 
15mm and numbered at one end. The strips were wetted halfway from the unlabelled end 
by immersion in absolute methanol for 15sec. Wetted strips were immediately transferred 
into distilled water and later stored in 1:256 dilution o f  methanol and distilled water.
Stored strips were retrieved and incubated in test urine samples for 30min at room 
temperature. The strips were rinsed in excess TBS (50mM Tris, 200mM NaCI, pH 7.0) 
and then blocked for 5min in 35% skimmed milk in TBS. Control strips not incubated in 
test urine were also blocked. After incubation the strips were washed three times in TBS 
and transferred into combined reagents consisting o f  MoAb and goat anti-mouse HRPO 
conjugate in TBS containing 0.1% skimmed milk for 1 hour with gentle rocking. They 
were then washed three times (lOmin/ wash) in excess TBS with gentle shaking on a 
rocker and then developed by incubation for lmin in substrate solution containing 0.025g 
diaminobenzidine tetrahydrochloride, 300]nl cobaltous chloride and 30^1 35% H2O2 in 
50jj.1 o f  TBS. Developed strips were immediately rinsed three times with excess distilled 
water to remove substrate. A bluish-black reaction represented positive results while 
negative results remained colourless. Control strips were used to assess the background 
and the test strips graded based on colour intensity.
Microplate-based Sandwich ELISA
Flat-bottomed Sero-wel micro-titre plates previously coated with MoAbs were 
washed twice with washing buffer and incubated for lh r with schistosome infected human 
urine samples. The plates were subsequently washed twice and the wells incubated (50jil/ 
well) for 30 min with HRPO-conjugated MoAbs diluted at 1:500 in blocking solution. 
After incubation they were washed further by flooding three times (lOmin/ wash) to 
remove unbound conjugates. The presence o f  the bound conjugate was revealed by the
addition o f 100(j.l o f substrate solution in each well and the plates kept in the dark for
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30min. Optical densities were read at 415nm wavelength using an MTP-32 micro plate 
reader (Corona Electric, Japan).
Membrane-based sandwich ELISA
The ability o f  the test MoAbs to capture schistosome antigen in membrane-based 
sandwich ELISA was assessed using PBS coating buffer at pH o f 7.4. PVDF strips, each 
coated with 2|j.l o f a test MoAb in dots was air dried. The strips were incubated in 
blocking solution (0.3% w/v casein) for 30 min with gentle shaking and then incubated in 
schistosome infected human urine for 1 hr. They were then washed twice in washing 
buffer (PBS pH 7.4, 0.1% Triton X-100) and incubated with MoAb-enzyme (HRPO) 
conjugate for 1 hr. After incubation the strips were further washed three times (10 
min/wash) in washing buffer and incubated in substrate solution (25ml TBS, pH 7.4; 
0.005g DAB; 150|il cobaltous nitrite; 15(il H2O2) for 1 min before they were transferred 
into distilled water.
Microscopical Diagnostic Methods
Collection and Analysis o f  Human Urine and Stool Specimen
Urine and stool specimens were collected from primary school pupils in Galilea 
between 11.00 and 14.00 hours. The samples were transported on ice to the laboratory. 
Ten millilitres o f  each urine sample was filtered through a 25mm nucleopore filter (12fim 
pore size) secured in a Swimnex support chamber. The filter membrane was removed with 
forceps and the side with trapped eggs laid face down on a labelled microscope slide. The 
urine filtrate was used for dipstick assay whilst excess unfiltered urine was centrifuged at 
l,290Xg for 5 min to sediment any schistosome eggs. The prepared slide and urine 
sediments were examined separately for schistosome eggs by microscopy. A drop of 
saline was placed on the filter to improve the refractive index.
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To detect parasitic infections by the Kato-Katz technique (Katz et al., 1972), a stool 
sample was taken with wooden spatula and forced through a stainless steel mesh to remove 
particulate and fibrous materials. The specimen was applied to fill a hole in a template set 
on a glass microscope slide, and the template carefully lifted to leave an intact plug o f 
faeces. This was then covered with a 25x2mm cellophane cover slip previously 
impregnated with 50% (v/v) glycerol in water containing 3% malachite green. The slide 
was subsequently turned face down on a flat surface and pressed gently but firmly to 
spread the stool specimen evenly. Prepared slides were left for 30min in the light to clear 
before microscopical examination for parasite eggs.
Collection and Analysis o f Cattle Blood and Faecal Samples
Blood and faecal samples o f cattle (West African short horn breed) were collected 
from Agbekotsekpo in the Dangbe West District o f the Greater Accra region. After 
collection, the blood samples were allowed to stand for 4 hours at room temperature and 
then kept at 4°C overnight to allow for maximum clotting. The samples were spun at 
2,500xg and the supernatant (serum) collected and stored at -20°C until needed.
The faecal samples were analysed by microscopy. Three grammes o f faeces was 
weighed into a beaker and 10ml o f  distilled water added to the sample and homogenised. 
The homogenised faeces was passed through a series o f  5 sedimentation sieves with 
stirring and the material left on the sieve washed with distilled water. The debris was 
discarded and the filtrate transferred into a conical flask and allowed to stand for 2 min. 
The supernatant was decanted and the remaining sample suspension transferred into a 
volumetric flask. This was allowed to sediment for 2min and the supernatant discarded. 
Few drops o f  5% methylene blue was added to the suspension and then observed under a 
microscope at 20x magnification for parasite ova.
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Fixation of miracidia with Karnovsky reagent
Miracidia were hatched from S. haematobium eggs obtained from urine o f infected 
individuals. The positive urine samples were pooled and spun at 500xg for 5min. The 
pellets containing the eggs were resuspended with a small volume o f water <5ml and 
transferred into filtered pond water in a volumetric flask using a pipette. Care was taken to 
deposit the egg suspension at the bottom o f the flask, which was then covered with 
aluminium foil up to the neck region. The contents o f  the flask was topped with water up 
to a level above the covered portion and placed in front o f a light source. The miracidia 
hatched from the eggs were attracted to the light and concentrated in a small volume o f 
exposed water. These were harvested with Pasteur pipette, chilled to 4°C and spun at 
2350xg for lOmin to concentrate the miracidia. Equal volume o f 4% Karnovsky reagent 
containing paraformaldehyde and glutaldehyde in PBS, pH 7.4 was added to the miracidia 
suspension to make a final concentration o f 2% Karnovsky reagent. This was incubated at 
4°C for 2 hours to fix the miracidia. The fixed miracidia was spun at 2,350xg for lOmin at 
4°C and washed 3 times with PBS by centrifugation. Miracidia were counted to estimate 
the concentration and stored in PBS 4°C until use.
IF AT Procedure
Twenty-four microlitres o f miracidia suspension was pipetted into a 1.5ml 
eppendorf tube and 1 |il bovine serum added to make a final concentration o f 1:25 dilution 
o f the serum. The mixture was incubated for 1 hour at room temperature with shaking at 5 
min interval. Dulbecco’s phosphate buffered saline (DPBS) was added and washed by 
centrifugation at 4,700xg for 10 min. It was then incubated for 30 min with 1:50 dilution 
o f anti-bovine FITC conjugate containing 0.01% trypan blue as counter stain. After 
incubation the mixture was washed three times by centrifugation at 4700xg for 10 min. 
The pellet was resuspended in 20fxl o f DPBS and I Ojj.1 o f the suspension observed using
fluorescent microscope (Olympus Optical Co. Ltd, Japan) at x400 magnification.
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CHAPTER 3
RESULTS 
Prepared monoclonal antibody reagents
Five hybridoma cell lines secreting Schistosoma genus-specific monoclonal 
antibodies (Sh3/34.10, Sh3/38.2, Sh4/14.3, Sh5/34.10 and Sh5/32.30) were selected from a 
panel o f 200 MoAbs generated at the Parasitology Unit of the NMIMR. Table 1, 
summarizes data on the type o f monoclonal antibody fractions used, their isotypes as 
determined by Double immunodiffusion, and the biochemical nature of the antigenic 
epitopes detected. With the exception o f Sh4/14.3, which is an IgGl, all the other 
monoclonal antibodies were o f IgM class.
Plate 1 presents a photograph showing a precipitin line used to identify the subclass 
o f Sh4/14.3 in Double immunodiffusion. The isotypes o f the other monoclonal antibodies 
were determined similarly as summarised in Table 1.
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Table 1. Some biochemical characteristics of the selected monoclonal antibodies
Monoclonal antibody Antibody fraction Isotype Nature of epitope *
Sh3/34.10 Purified b IgM Protein
Sh3/38.2 Purified b IgM Carbohydrate/protein
Sh4/14.3 Amicon conc.c IgGl Protein
Sh5/32.30 Purified b IgM Protein
Sh5/34.10 Purified b IgM Protein
“Biochemical characteristics o f the epitope bound by monoclonal antibody [after, Yeboah (1998) M.Phil 
thesis University o f Ghana, Legon].
bIgM monoclonal antibody fraction purified by gel filtration.
c Monoclonal antibody in culture supernatant concentrated 30 fold by amicon filtration.
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Plate I Photograph showing precipitin lines (indicated by arrows) used 
to identify the subclass of Sh4/14.3 in double immunodiffusion
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Reactivity of selected monoclonal antibodies as determined by micro-plate ELISA
The suitability o f the selected anti-schistosome monoclonal antibodies (Sh3/34.10, 
Sh3/38.2, Sh4/14.3, Sh5/34.10 and Sh5/32.30) as diagnostic reagents was determined by 
their ability to specifically detect Schistosoma genus-specific antigens. As shown in Table 
2, there was reactivity between the antibodies and the different schistosome antigens used. 
The genus-specificity o f the MoAbs was confirmed using antigens o f  S. haematobium, S. 
mansoni, and S. japonicum  by microplate ELISA.
Cross-reactivity analysis of the selected anti-schistosome monoclonal antibodies 
with P. falciparum  crude antigen extract and circum-sporozoite antigen was determined. 
The results are also presented in Table 2. As shown, none o f  the test monoclonal 
antibodies could react with the circum-sporozoite antigens. However, two o f the 
monoclonal antibodies (Sh3/34.10 and Sh5/34.10) reacted with the P. falciparum  crude 
antigen extract at higher MoAb concentrations (Figures 1-5) even though the reactivity 
declined sharply to OD < 0.1 at lower concentrations (dilution >1:100). On the other hand, 
the reactivity o f  Sh3/34.10 and Sh5/34.10 with the schistosome antigens remained high at 
all the dilutions tested (Figures 1 and 5).
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Table 2. Reactivity of the selected monoclonal antibodies with Schistosoma 
species and Plasmodium falciparum  antigens
MoAb Reactivity o f monoclonal antibodies with 
antigens o f  different schistosome species
Reactivity o f  monoclonal 
antibodies with P. falciparum  
antigens
S.
haematobium
S. mansoni S. japonicum Circum-
sporozoite
antigen
Crude antigen 
extract2
Sh3/34.10 + + + +
Sh3/38.2 + + + -
Sh4/14.3 + + + -
Sh5/32.30 + + + - -
Sh5/34.10 + + + - +
“Crude antigen extract of different P. falciparum  life cycle stages obtained from culture.
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O
pt
ic
al
 d
en
si
ty
 
at 
41
5n
m
MoAb dilution
Figure 1. Reactivity of Sh3/34.10 with schistosome antigen and P. falciparum
crude antigen extract at different MoAb dilutions
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Op
tic
al
 d
en
sit
y 
at 
41
5n
m
Neat 1:5 1:10 1:20 1:50 1:100 1:200 1:400 1:800 1:1600 1.3200
MoAb dilution
Figure 2. Reactivity of Sh3/38.2 with schistosome antigen and P. falciparum  
crude antigen extract at different MoAb dilutions
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Op
tic
al
 d
en
sit
y 
at 
41
Bn
m
Neat 1:5 1:10 1:20 1:50 1:100 1 200 1:400 1 800 1 1600 1:3200
MoAb dilution
Figure 3. Reactivity of Sh4/14_3 with schistosome antigen and P. falciparum
crude antigen extract at different MoAb dilutions
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Figure 4. Reactivity of Sh5/32.30 with schistosome antigen and P. falciparum  
crude antigen extract at different MoAb dilutions
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Figure 5. Reactivity of Sh5/34.10 with schistosome antigen and P. falciparum  
etude antigen extract at different MoAb dilution
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Development of assays
Detection o f Schistosoma antigens in human urine using the selected monoclonal 
antibodies
Table 3 summarises results o f microscopic identification o f parasite ova in human 
urine and the ability o f the selected monoclonal antibodies to detect Schistosoma antigens 
when evaluated using the standard dipstick-ELISA protocol. The result obtained with 
Sh2/15.F, the monoclonal antibody utilized in the standard urinary schistosomiasis 
dipstick-ELISA, was used as the basis to assess the other monoclonal antibodies. Out o f 
74 urine samples examined, Sh2/15.F detected antigen in 65 (87.8%) (Table 4), and 
microscopy revealed S. haematobium ova in 60/65 (92.3%) o f  them (Table 3). The five 
Schistosoma genus-specific monoclonal antibodies (Sh3/34.10, Sh3/38.2, Sh4/14.3, 
Sh5/32.30 and Sh5/34.10) detected antigen in different numbers o f the infections identified 
by the standard Sh2/15.F dipstick-ELISA (Table 3). As shown, they recorded 
comparatively lower relative sensitivities (ranging from 60.0 to 71.7%) when compared 
with microscopy as the gold standard test (Table 3). There were no significant differences 
(p<0.05) in relative sensitivities o f the assays utilizing the different Schistosoma genus 
specific MoAbs in detecting schistosome antigens. However they were significantly 
different from the performance o f the standard Sh2/15.F dipstick-ELISA, which gave a 
relative sensitivity o f  100%. Interestingly, each o f  the Schistosoma genus-specific MoAbs 
detected schistosome antigens in only urine samples, which were microscopically positive, 
thereby indicating 100% specificity. On the other hand the standard Sh2/15.F dipstick- 
ELISA recorded a specificity o f 64.3% (9/14). As shown in Table 5, the S. haematobium 
egg positive samples detected by the dipstick assays utilizing the selected MoAbs had 
intensities ranging from 2-3000 eggs/10ml urine (median = 295, mean = 498), however the 
egg positive samples not correctly detected by the different assays had overall egg count 
ranging from 50-2800 eggs/10ml urine (median = 274, mean = 492). Each o f  the dipstick
assays failed to detect some infections within egg count ranges that were revealed in other
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subjects. O f the different dipstick assays, Sh3/34.10, Sh5/32.30 andSh5/34.10 detected 
antigens in the widest range o f egg counts. Assays utilizing MoAb Sh4/14.3 detected 
infections involving the minimum number o f  egg counts.
Using urine samples o f  individuals who were infected with S. mansoni, the ability 
o f  the selected monoclonal antibodies to detect S. mansoni antigen was evaluated by 
dipstick-ELISA. Microscopic analysis revealed that 44 out o f 55 (80.0%) individuals 
examined were S. mansoni egg positive, and 40/44 (90.9%) had mixed infections with S. 
haematobium (Table 3). This gave a prevalence o f 72.7% for mixed infections involving 
S. mansoni and S. haematobium. With the exception o f S. mansoni, no other human 
intestinal parasite ova were detected. The relative sensitivity o f the different Schistosoma 
genus-specific MoAbs in detecting S. mansoni infections, using microscopy as gold 
standard test ranged from 61.3% to 63.6% (Table 3). However, the differences in 
sensitivity o f the various assays were not significant (p>0.05). On the other hand, the 
relative sensitivity o f the Sh2/15.F based-dipstick recorded a higher sensitivity o f  95.5% 
(42/44). As shown in Table 3, 40 out o f the 42 Sh2/15.F-dipstick positives were also 
confirmed to be infected with S. haematobium by demonstration o f  the parasite’s eggs. 
Interestingly, Sh2/15.F dipstick-ELISA detected antigens in 2/4 (50%) o f single infections 
involving S. mansoni as determined by microscopy. None o f  the selected genus-specific 
MoAbs could detect antigens in single infections involving S. mansoni.
60
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63
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Ability o f the selected MoAbs to coat onto different micro-titre plates and membranes
Table 6 shows the ability o f the selected MoAbs to bind onto different micro-titre 
plates [sero-wel (Cat No. 612F96), sero-well (Cat. No. 611U96), sumilon (Ms-8496F)] and 
membranes [PVDF (Cat No. 1PUH20200) and nitrocellulose (Cat No. 13H0457)]. MoAb 
coated plates were probed using goat anti-mouse immunoglobulin HRPO conjugates and 
revealed with ABTS substrate. As shown in table 6 all the MoAbs (Sh3/34.10, Sh3/38.2, 
Sh4/14.3, Sh5/32.30 and Sh5/34.10) could coat onto the three different micro-titre plates 
tested. However, the assessment o f binding based on colour intensity showed that the 
MoAbs were better retained by the sero-wel (Cat No. 612F96) plate, followed by Sumilon 
before sero-well (Cat. No. 611U96). Sero-well (Cat No. 612F96), which exhibited the 
highest binding o f MoAbs, was therefore selected for further experiments to detect 
schistosome antigens in human urine.
Investigation into the binding o f  the MoAbs to different membranes in dot-ELISA 
also revealed that the antibodies could bind to both membranes (Table 6). Bound 
antibodies remained detectable in both membranes after extensive washing in PBS buffer. 
Both membranes showed higher MoAb binding at the highest, pH 7.4 compared to pH 7.0 
and pH 7.2 that were evaluated. The intensity o f  colour development was however higher 
on PVDF (Table 6). The PVDF membrane was therefore used in the subsequent assays.
64
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Detection o f schistosome antigens in human urine using the selected monoclonal
antibodies in sandwich ELISA
Following the successful detection o f schistosome antigens in infected human urine 
using the selected MoAbs in dipstick ELISA, experiments were conducted to capture the 
antigens in sandwich ELISA utilizing micro-titre plates and membranes coated with the 
MoAbs. Interestingly, none of the selected MoAbs could demonstrate captured 
schistosome antigen when used along side its own enzyme-conjugate in a homologous 
ELISA.
Prevalence of Schistosoma infection in cattle as determined by microscopy
In order to identify cattle infected with schistosomes, faecal specimens from 32 
animals were screened by microscopy. As shown in Table 7, ova o f  Schistosoma bovis 
were identified in 17 (53.1%) o f  the faecal specimen examined. Also, one specimen 
(3.1%) was positive for S. indicum eggs. Typical S. bovis eggs found are shown in Plate 2. 
In addition to the schistosome infections, other cattle parasites were identified (Table 7). 
The prevalence o f  the other infections ranged from 3.1% to 21.9% (Table 7). Interestingly, 
each o f  the 32 faecal samples examined showed the presence o f at least one parasite 
infection.
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Table 7 Detection of parasite ova in stool samples of cattle (short horn variety) 
by microscopy from Agbekpotsepko
Parasite Number o f  stool 
samples examined
Number o f  cattle 
infected
Prevalence
%
Schistosoma bovis 32 17 53.1
Schistosoma indicum 32 1 3.1
Mecistocirrus digitatus 32 5 16.0
Eimeria aubumensis 32 5 15.6
Eimeria subspherica 32 7 21.9
Syngamus laryngeus 32 1 3.1
Eimeria zumii 32 5 15.6
Oesophagostomum radialum 32 5 15.6
Trichostrongylus axei 32 7 21.9
Ascaris vitulorum 32 1 3.1
Bonustomum phlebotomum 32 1 3.1
Cooperia sp 32 1 3.1
Fasciola 32 4 12.5
67
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Schistosoma infection rates in cattle as determined by IF AT and micro-plate ELISA
Schistosome infections in cattle were also diagnosed by detection o f  anti­
schistosoma antibodies using IFAT, or antigen using micro-plate ELISA. Out o f 32 cattle 
sera screened, 16 tested positive for schistosome antibodies, giving a seroprevalence o f  
50%. The sero-positives included 16 o f the 17 microscopically confirmed schistosome 
infections in the cattle (94.1%).
The ability o f  the selected MoAbs to detect schistosome antigens in cattle sera was 
assessed using micro-plate ELISA protocol. The different MoAbs detected antigens in 
sera of cattle confirmed to be infected with S. bovis by microscopy. They recorded 
different relative sensitivities (ranging from 46.8 to 50.0%) when compared with 
microscopy as the gold standard test (Table 8). However, there were no significant 
differences (p>0.05) in relative sensitivities o f the assays. All the antigen positive sera 
were also positive for anXx-Schistosoma antibodies as determined by IFAT.
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Table 8 Diagnosis of schistosomiasis in cattle by microscopy and micro-plate
ELISA using the selected MoAbs
MoAb No o f sera 
examined
Microscopy
positve
Plate-ELISA
positive3
Relative 
sensitivityb (%)
Prevalence
(%)
Sh3/34.10 32 17 15 88.2 46.9
Sh3/38.2 32 17 16 94.1 50.0
Sh4/14.3 32 17 16 94.1 50.0
Sh5/32.30 32 17 15 88.2 46.9
Sh5/34.10 32 17 15 88.2 46.9
“ Number of sera samples testing positive for schistosome antigens in micro-plate ELISA 
utilising the different MoAbs. 
b Sensitivity of Plate-ELISA assays utilising the different MoAbs as compared to microscopical 
detection of
schistosome egg as gold standard.
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CHAPTER FOUR 
DISCUSSION AND CONCLUTION
The objective o f  the series o f experiments described in this thesis was to evaluate 
the diagnostic potential o f selected anti-Schistosoma genus-specific MoAbs (Sh3/34.10, 
Sh3/38.3, Sh4/14.3, Sh5/32.30 and Sh5/34.10) in detection o f S. mansoni in humans and 
Schistosoma species in animals. The strategy was to purify the MoAbs, determine their 
reactivity and utilize them in diagnosis o f schistosomiasis, whilst comparing with the 
established urinary schistosomiasis dipstick (Bosompem et al., 1998).
Analysis o f culture supernatants from the selected hybridoma cell lines in this study 
revealed the presence o f  MoAbs of IgG and IgM isotypes which were also confirmed to 
react with schistosome antigens. In a previous study Yeboah (1996), reported the lack of 
cross reactivity o f  the MoAbs (Sh3/34.10, Sh3/38.3, Sh4/14.3, Sh5/32.30 and Sh5/34.10) 
with antigens o f Necator americanus a common endemic parasite in Ghana. In this study, 
the specificity o f three o f  the selected MoAbs (Sh3/38.3, Sh4/14.3 and Sh5/32.30) with 
schistosome antigens was further demonstrated by the lack o f cross reactivity with antigens 
o f the highly endemic malaria parasite P. falciparum. It is therefore unlikely that the 
presence o f hookworm and/or P. falciparum  infections would influence the results o f  any 
assays developed with these MoAbs. However two o f the MoAbs, Sh3/34.10 and 
Sh5/34.10 reacted with crude antigen extract o f  P. falciparum  at high MoAbs 
concentrations, suggesting that these MoAbs could only be utilized in diagnosis at high 
antibody titres where cross-reactivity did not occur; even though the sensitivity o f the 
assays developed could be compromised.
The diagnostic potential o f the selected Schistosoma genus-specific MoAbs was 
first assessed using S. haematobium infected human urine samples. This approach was 
thought feasible because o f two reasons. Firstly, as a species o f the Schistosoma genus, S.
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haematobium antigens were detected by each o f the MoAbs. Secondly, the more sensitive 
urinary schistosomiasis dipstick assay (Bosompem et al., 1996a, 1997, 1998) was available 
to be used alongside microscopy to facilitate the assessment. Interestingly, the urinary 
schistosomiasis prevalence estimated by the established Sh2/15.F MoAb-based urinary 
schistosomiasis dipstick (87.8%) was not statistically different (p>0.05) from that o f 
microscopy (81.1%). However, the assays utilizing the selected MoAbs gave significantly 
lower prevalence estimates (48.6-58.1%) than either microscopy or the urinaiy 
schistosomiasis dipstick, indicating that the developed assays were less sensitive. 
Furthermore, the higher relative sensitivity (100%) recorded by the urinary schistosomiasis 
dipstick compared to that o f the assays (60.0-71.1%) utilizing the selected Schistosoma 
genus-specific MoAbs suggested that the established dipstick was more sensitive in 
detecting S. haematobium infections in humans. However, this may not be true when the 
same MoAbs are utilized in assays based on principles other than that of the urinary 
schistosomiasis dipstick. This is because the urinary schistosomiasis dipstick is based on 
random binding o f  antigens in urine onto a membrane and then probed with specific 
antibodies. This could be less sensitive than assays based on selective binding o f antigen 
by membrane coated antibodies. This notwithstanding, the specificity o f the assays 
developed with the selected MoAbs was each 100% compared with the urinary 
schistosomiasis dipstick, which gave a specificity o f  64.3%. In earlier studies Bosompem 
et al, 1997 observed that the high sensitivity o f the Sh2/15.F MoAb-based urinary 
schistosomiasis dipstick gave a corresponding lower specificity when compared with 
microscopy as the gold standard test.
The inability o f the developed genus-specific dipstick assays to detect some
microscopically confirmed infections did not appear to be associated with a particular
intensity o f infection (low or high) as determined by egg count analysis. The mean egg
count of microscopically confirmed infections detected by the dipstick assays was 498
egg/10ml urine. This was not significantly different from the mean egg count (492
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egg/10ml) o f  microscopically confirmed infections that were not detected by the MoAb 
dipstick assays. In a previous study Bosompem et al, 1998 reported that the failure of 
urinary schistosomiasis dipstick-ELISA to detect known S. haematobium infections was 
likely to be due to peculiar immunological reactions. They emphasised that schistosome 
antigens occur in infected human urine mainly as immune complexes together with human 
immunoglobulins and complement, possibly leading to masking o f  diagnostic epitopes 
during the course o f  infection. There is the likelihood that the same phenomenon underlies 
the observation in the present study. Investigations into the pre-treatment o f urine samples 
to dissociate immune complexes in order to improve sensitivity should therefore be 
pursued.
The suitability o f  the genus-specific MoAbs to detect Schistosoma antigens was 
further assessed using S. mansoni infected human urine specimens. Similar to the 
observation made in the diagnosis o f S. haematobium infection using the Schistosoma 
genus-specific MoAb-based dipstick assays, the estimated prevalences (49.1-50.1%) o f  S. 
mansoni infections were statistically lower (p<0.05) than that by microscopy (80.0%). 
Furthermore, the developed assays recorded significantly lower relative sensitivities (61.3­
63.6%) compared with microscopy as the gold standard test. The dipstick assay could 
detect antigens in single infections involving S. haematobium and mixed infections 
involving S. haematobium and S. mansoni. The failure o f  the dipstick assays to detect 
infections involving only S. mansoni may suggest that the genus-specific antibodies are 
incapable o f detecting S. mansoni infections. However, the small number (4/44) o f S. 
mansoni single infections involved makes it difficult to draw conclusions, and the ability 
o f the antibodies to detect S. mansoni antigens in vitro suggests that this may not be the 
case.
Bosompem et al. (1997; 1998) emphasized the need for repeated urine examination 
to identify low intensity S. haematobium infections by microscopy. The observation that
urine samples from two S. mansoni infected individuals in this study were positive for
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antigen by the urinary schistosomiasis dipstick assay was therefore not surprising. This is 
because concomitant S. haematobium infection could be missed by microscopy without 
repeated testing. Furthermore, Amanor et al. (1996), observed that the MoAb (Sh2/15.F) 
utilized in the urinary schistosomiasis dipstick did not cross-react with S. mansoni 
antigens.
In this study, successful coating o f each o f  the selected MoAbs onto solid support 
provided an opportunity for the antibodies to be utilized in sandwich ELISA. Studies have 
shown that the sandwich ELISA is one o f  the most sensitive and specific assay systems in 
immunodiagnosis (Chi Fu and Cater, 1990; Barsoum et al., 1991). However, none o f the 
MoAbs investigated could reveal antigens in both the plate- and membrane-based 
sandwich ELISA. One possible explanation for the inability o f the MoAbs to detect 
antigens in sandwich ELISA even though they detected antigens in direct ELISA is that the 
antigens possess single diagnostic epitopes. This may be because the sandwich ELISA 
requires that target antigens to have multiple epitopes that make it possible to use similar 
antibodies to capture and reveal the antigens. Hence the exploration o f the selected 
MoAbs to diagnose schistosomiasis in humans using sandwich ELISA technique was 
discontinued.
Development o f alternative diagnostic techniques for animal schistosomiasis was 
investigated using cattle. In a previous study, Boulanger et al. (1999) reported that S. bovis 
is one o f the main schistosome species affecting domestic ruminants in Africa o f which 
cattle is among the potential reservoirs. In highly endemic areas o f  human schistosomiasis, 
the possibility o f  identifying some species o f human schistosomes in animals such as cattle 
cannot be underestimated. For example, cattle and dogs could be naturally infected with S. 
mansoni and they are sources o f continual transmission (Mayaudontarbes and Power, 
1969; 1970; Nelson et al., 1962; Mango, 1971). The choice o f cattle in this study to 
investigate the importance of animal schistosomiasis was therefore justifiable.
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Analysis o f  cattle faeces for parasites by microscopy showed a high prevalence o f 
S. bovis. Rollinson and Southgate (1987) reported that this parasite is a serious veterinary 
problem. In Sudan a prevalence of nearly 90% in 18-month-old cattle was demonstrated 
by Majid et al. (1980). S. bovis is capable o f utilizing a wide variety o f Bulinus species as 
molluscan host, often developing naturally in snails o f B. truncates/tropicus, B. africanus 
and B. forskalii group (Southgate and Knowles, 1975), which may also be the intermediate 
hosts for the human schistosomes. It is not surprising therefore that S. bovis is reported to 
incidentally infect man (Rollinson and Southgate, 1987). The relatively high prevalence 
(53.1%) o f S. bovis found in this study may not rule out the possibility o f  incidental 
infections in the local population. Interestingly, the prevalence o f S. bovis by microscopy 
was not significantly (p>0.05) higher than the 50.0% prevalence obtained using the newly 
developed IFAT. Likewise, the newly developed Schistosoma genus-specific MoAb-based 
plate-ELISAs estimated prevalences (46.9-50.0%) that were not statistically lower than 
that o f  microscopy. The high sensitivity (94.1%) and specificity (100%) o f the IFAT 
clearly indicated its potential as an alternative diagnostic tool for detecting schistosomes in 
cattle. Also, the MoAb-based plate-ELISAs utilizing (Sh3/38.2 and Sh4/14.3) had high 
attributes, 100% specificity and 94.1% relative sensitivity in detecting S. bovis in cattle. 
This work has therefore established two possible assays (IFAT and plate-ELISA) as 
potential alternatives to microscopic diagnosis o f  schistosomiasis in cattle. There is an 
urgent need to further evaluate these tests in order to adopt one for routine diagnosis of 
animal schistosomiasis, preferably in the field. The use o f  ELISA as a screening test is 
justified, considering its advantages over other methods o f  diagnosis. It is highly sensitive, 
specific, non-hazardous to technicians, can be semi-automated and quantitative (Waltman 
et al., 1984; Hirvela-Koski, 1990). However it has been explained that IFAT utilises 
whole cells o f parasites, while the antigen for ELISA consists o f  soluble proteins. IFAT is 
therefore able to detect antibodies which appear at the early stage o f infection against
antigenic components of the intact parasites (Karim and Ludlam, 1975), whereas ELISA is
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better suited for detecting antigens that appear later in infection. The choice between IFAT 
and ELISA therefore could be influenced by the kind of diagnostic tool required. Thus, for 
example, a screening assay capable o f detecting early infections will be preferred in 
disease surveillance so as to enable early intervention. On the other hand, the ELISA is 
extremely economical in the use o f reagents (Riott et al., 1993) and large numbers o f tests 
can be performed in a relatively short time. It is therefore recommended that ELISA is 
developed for field diagnosis o f animal schistosomiasis whilst IFAT is used for 
confirmatory purposes in the laboratory.
The study also demonstrated 3.1% prevalence o f  S. indicum in mixed infections 
with S. bovis. In India, S. indicum is known to infect a variety o f domesticated animals 
including sheep, camel, goat buffalo and cattle (Rollinson and Southgate, 1987). It is 
known to be among the veterinary schistosomes which are o f less medical importance 
because its range is free o f human schistosomes (Chandler, 1926). However, it is known 
that cercariae o f many non-human schistosomes penetrate man but die in the skin. Such 
infections are not usually significant but can cause a cercarial dermatitis referred to as 
swimmers itch and repeated exposure may lead to a severe allergic reaction (Macfarlane, 
1949; Olivier, 1949). The observation o f  bovine schistosomiasis in parts o f Ghana where 
human schistosomiasis is known to be endemic is therefore important. It is expected that 
the information would be useful as a basis to launch a thorough investigation into animal 
schistosomiasis, which has previously received little attention in Ghana.
Even though eleven other cattle parasites were identified by microscopy, none o f 
them showed cross-reactivity with the MoAbs used. This is because none o f the sera from 
the Schistosoma negative animals was positive for antigen by the MoAb-based micro-plate 
ELISA, indicating a 100% specificity o f  the assays.
In conclusion, alternative assays (micro-plate ELISA and IFAT) have been 
developed and shown to be highly sensitive and specific in detecting Schistosoma
infections in cattle. The assays are likely to contribute towards better understanding o f the
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distribution and interactions o f the animal schistosomiases in Ghana, and thereby create 
opportunities to explore zoonotic schistosomiasis in the country.
In the case o f  human schistosomiasis, the established S. haematobium species- 
specific dipstick (Bosompem et al., 1998) proved to be sensitive in detecting urinary 
schistosome antigens. On the other hand, the lower sensitivities recorded by the newly 
developed Schistosoma genus-specific dipstick assays even though the specificities were 
very high, underscore the need to explore the MoAbs in different assay systems.
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